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BSTA: a targeted approach combines bulked segregant analysis with next- generation sequencing and de novo transcriptome assembly for SNP discovery in sunflower

机译:BSTA:一种有针对性的方法将大量的分离子分析与下一代测序和从头转录组组装相结合用于发现向日葵中的SNP

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摘要

BackgroundSunflower belongs to the largest plant family on earth, the genomically poorly explored Compositae. Downy mildew Plasmopara halstedii (Farlow) Berlese & de Toni is one of the major diseases of cultivated sunflower (Helianthus annuus L.). In the search for new sources of downy mildew resistance, the locus PlARG on linkage group 1 (LG1) originating from H. argophyllus is promising since it confers resistance against all known races of the pathogen. However, the mapping resolution in the PlARG region is hampered by significantly suppressed recombination and by limited availability of polymorphic markers. Here we examined a strategy developed for the enrichment of molecular markers linked to this specific genomic region. We combined bulked segregant analysis (BSA) with next-generation sequencing (NGS) and de novo assembly of the sunflower transcriptome for single nucleotide polymorphism (SNP) discovery in a sequence resource combining reads originating from two sunflower species, H. annuus and H. argophyllus.
机译:背景向日葵属于地球上最大的植物科,在基因组学上探索不佳的菊科。霜霉病Plasmopara halstedii(Farlow)Berlese&de Toni是栽培向日葵(Helianthus annuus L.)的主要疾病之一。在寻找霜霉病抗性的新来源中,起源于argophyllus的连锁群1(LG1)上的PlARG基因座很有希望,因为它赋予了对病原体所有已知种族的抗性。然而,PlARG区域中的作图分辨率受到明显​​抑制的重组和多态性标记物有限可用性的阻碍。在这里,我们检查了为丰富与该特定基因组区域相关的分子标记而开发的策略。我们将批量隔离分析(BSA)与下一代测序(NGS)和向日葵转录组的从头组装相结合,以用于在序列资源中发现源自两个向日葵物种H. annuus和H的读段的单核苷酸多态性(SNP)。 Argophyllus。

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