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首页> 外文期刊>BMC Evolutionary Biology >A genome-scale mining strategy for recovering novel rapidly-evolving nuclear single-copy genes for addressing shallow-scale phylogenetics in Hydrangea
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A genome-scale mining strategy for recovering novel rapidly-evolving nuclear single-copy genes for addressing shallow-scale phylogenetics in Hydrangea

机译:基因组规模的采矿策略,用于恢复新型快速进化的核单拷贝基因,以解决绣球花的浅层系统发育问题

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Background Identifying orthologous molecular markers that potentially resolve relationships at and below species level has been a major challenge in molecular phylogenetics over the past decade. Non-coding regions of nuclear low- or single-copy markers are a vast and promising source of data providing information for shallow-scale phylogenetics. Taking advantage of public transcriptome data from the One Thousand Plant Project (1KP), we developed a genome-scale mining strategy for recovering potentially orthologous single-copy markers to address low-scale phylogenetics. Our marker design targeted the amplification of intron-rich nuclear single-copy regions from genomic DNA. As a case study we used Hydrangea section Cornidia, one of the most recently diverged lineages within Hydrangeaceae (Cornales), for comparing the performance of three of these nuclear markers to other “fast” evolving plastid markers. Results Our data mining and filtering process retrieved 73 putative nuclear single-copy genes which are potentially useful for resolving phylogenetic relationships at a range of divergence depths within Cornales. The three assessed nuclear markers showed considerably more phylogenetic signal for shallow evolutionary depths than conventional plastid markers. Phylogenetic signal in plastid markers increased less markedly towards deeper evolutionary divergences. Potential phylogenetic noise introduced by nuclear markers was lower than their respective phylogenetic signal across all evolutionary depths. In contrast, plastid markers showed higher probabilities for introducing phylogenetic noise than signal at the deepest evolutionary divergences within the tribe Hydrangeeae (Hydrangeaceae). Conclusions While nuclear single-copy markers are highly informative for shallow evolutionary depths without introducing phylogenetic noise, plastid markers might be more appropriate for resolving deeper-level divergences such as the backbone relationships of the Hydrangeaceae family and deeper, at which non-coding parts of nuclear markers could potentially introduce noise due to elevated rates of evolution. The herein developed and demonstrated transcriptome based mining strategy has a great potential for the design of novel and highly informative nuclear markers for a range of plant groups and evolutionary scales.
机译:背景技术在过去的十年中,鉴定可能解决物种水平及低于物种水平的关系的直系同源分子标记一直是分子系统发生学中的主要挑战。核低拷贝或单拷贝标记的非编码区是一个广阔而有希望的数据来源,可为浅层系统发育学提供信息。利用千植物计划(1KP)的公共转录组数据,我们开发了一种基因组规模的挖掘策略,用于回收潜在的直系同源单拷贝标记,以解决低尺度的系统发育问题。我们的标记设计旨在从基因组DNA扩增富含内含子的核单拷贝区域。作为案例研究,我们使用了绣球花科尼迪亚科(绣球科(Cornales)中最近分化的血统)之一,将这三种核标记与其他“快速”进化的质体标记的性能进行了比较。结果我们的数据挖掘和过滤过程检索了73个推定的核单拷贝基因,这些基因对于解决Cornales内一系列发散深度的系统发育关系可能有用。与传统的质体标记相比,这三个评估的核标记在浅的进化深度上显示出更多的系统发生信号。质体标记中的系统发生信号向更深的进化差异显着增加。在所有进化深度上,由核标记引入的潜在系统发生噪声均低于其各自的系统发生信号。相比之下,质体标记显示的系统发生噪声的概率要高于绣球部落(绣球科)内最深的进化分歧处的信号。结论虽然核单拷贝标记物在不引起系统发育噪声的情况下对于浅层进化深度具有很高的信息价值,但质体标记物可能更适合解决更深层次的分歧,例如绣球花科的骨干关系以及更深层次的分歧,而在这种情况下,绣球花科的非编码部分核标记物可能会因进化速度加快而引入噪音。本文开发和证明的基于转录组的挖掘策略对于设计用于一系列植物群和进化规模的新颖且高度有用的核标记物具有巨大潜力。

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