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通过 RAD 测序和连锁图谱构建到斑胸草雀基因组,在一种非模式雀形目鸟类中大规模生产 SNP 标记。

Mass production of SNP markers in a nonmodel passerine bird through RAD sequencing and contig mapping to the zebra finch genome.

机构信息

Laboratoire Évolution et Diversité Biologique, UMR 5174 CNRS - Université Paul Sabatier - ENFA, 118 route de Narbonne, Bâtiment 4R1, F-31062, Toulouse Cedex 9, France.

出版信息

Mol Ecol Resour. 2013 Sep;13(5):899-907. doi: 10.1111/1755-0998.12137. Epub 2013 Jul 16.

Abstract

Here, we present an adaptation of restriction-site-associated DNA sequencing (RAD-seq) to the Illumina HiSeq2000 technology that we used to produce SNP markers in very large quantities at low cost per unit in the Réunion grey white-eye (Zosterops borbonicus), a nonmodel passerine bird species with no reference genome. We sequenced a set of six pools of 18-25 individuals using a single sequencing lane. This allowed us to build around 600 000 contigs, among which at least 386 000 could be mapped to the zebra finch (Taeniopygia guttata) genome. This yielded more than 80 000 SNPs that could be mapped unambiguously and are evenly distributed across the genome. Thus, our approach provides a good illustration of the high potential of paired-end RAD sequencing of pooled DNA samples combined with comparative assembly to the zebra finch genome to build large contigs and characterize vast numbers of informative SNPs in nonmodel passerine bird species in a very efficient and cost-effective way.

摘要

在这里,我们介绍了一种将限制性位点相关 DNA 测序 (RAD-seq) 改编为 Illumina HiSeq2000 技术的方法,我们使用该方法在没有参考基因组的非模式 passerine 鸟类 Réunion 灰眼鸟 (Zosterops borbonicus) 中以低成本大量产生 SNP 标记。我们使用单个测序通道对六组 18-25 个个体进行了测序。这使我们能够构建大约 600,000 个重叠群,其中至少 386,000 个可以映射到斑胸草雀 (Taeniopygia guttata) 基因组。这产生了超过 80,000 个可以明确映射的 SNP,并且均匀分布在基因组上。因此,我们的方法很好地说明了结合比较组装的成对末端 RAD 测序的潜力,可以有效地以低成本的方式在非模式 passerine 鸟类物种中构建大量重叠群并鉴定大量信息丰富的 SNP。

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