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A workflow of massive identification and application of intron markers using snakes as a model

机译:以蛇为模型大规模鉴定和应用内含子标记的工作流程

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摘要

Abstract Relative to the commonly used mitochondrial and nuclear protein-coding genes, the noncoding intron sequences are a promising source of informative markers that have the potential to resolve difficult phylogenetic nodes such as rapid radiations and recent divergences. Yet many issues exist in the use of intron markers, which prevent their extensive application as conventional markers. We used the diverse group of snakes as an example to try paving the way for massive identification and application of intron markers. We performed a series of bioinformatics screenings which identified appropriate introns between single-copy and conserved exons from two snake genomes, adding particular constraints on sequence length variability and sequence variability. A total of 1,273 candidate intron loci were retrieved. Primers for nested polymerase chain reaction (PCR) were designed for over a hundred candidates and tested in 16 snake representatives. 96 intron markers were developed that could be amplified across a broad range of snake taxa with high PCR successful rates. The markers were then applied to 49 snake samples. The large number of amplicons was subjected to next-generation sequencing (NGS). An analytic strategy was developed to accurately recover the amplicon sequences, and approximately, 76% of the marker sequences were recovered. The average p -distances of the intron markers at interfamily, intergenus, interspecies, and intraspecies levels were .168, .052, .015, and .004, respectively, suggesting that they were useful to study snake relationships of different evolutionary depths. A snake phylogeny was constructed with the intron markers, which produced concordant results with robust support at both interfamily and intragenus levels. The intron markers provide a convenient way to explore the signals in the noncoding regions to address the controversies on the snake tree. Our improved strategy of genome screening is effective and can be applied to other animal groups. NGS coupled with appropriate sequence processing can greatly facilitate the extensive application of molecular markers.
机译:摘要相对于常用的线粒体和核蛋白编码基因,非编码内含子序列是信息标记物的有希望的来源,其有可能解决困难的系统发育节点,例如快速辐射和最近的发散。内含子标记物的使用还存在许多问题,这阻碍了它们作为常规标记物的广泛应用。我们以不同种类的蛇为例,试图为大规模鉴定和应用内含子标记物铺平道路。我们进行了一系列生物信息学筛选,从两个蛇基因组中鉴定出单拷贝和保守外显子之间的适当内含子,并对序列长度变异性和序列变异性增加了特殊的限制。总共检索到1,273个候选内含子基因座。巢式聚合酶链反应(PCR)引物的设计是针对一百多种候选物,并在16个蛇代表中进行了测试。已开发出96种内含子标记,可在各种蛇类群中以高PCR成功率进行扩增。然后将标记物应用于49个蛇样品。对大量扩增子进行了下一代测序(NGS)。已开发出一种分析策略来准确回收扩增子序列,并回收了大约76%的标记序列。内含子标记在家族间,属间,种间和种内水平的平均p距离分别为.168,.052,.015和.004,这表明它们对于研究不同进化深度的蛇关系很有用。用内含子标记构建了系统发育的蛇,它在家族间和属内水平上都产生了一致的结果,并得到了强有力的支持。内含子标记提供了一种方便的方法来探索非编码区域中的信号,以解决蛇树上的争议。我们改进的基因组筛选策略是有效的,可以应用于其他动物群体。 NGS加上适当的序列处理可以极大地促进分子标记物的广泛应用。

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