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首页> 外文期刊>Genome Biology >Targeted analysis of nucleotide and copy number variation by exon capture in allotetraploid wheat genome.
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Targeted analysis of nucleotide and copy number variation by exon capture in allotetraploid wheat genome.

机译:通过异源四倍体小麦基因组中外显子捕获对核苷酸和拷贝数变异进行靶向分析。

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Background: The ability of grass species to adapt to various habitats is attributed to the dynamic nature of their genomes, which have been shaped by multiple rounds of ancient and recent polyploidization. To gain a better understanding of the nature and extent of variation in functionally relevant regions of a polyploid genome, we developed a sequence capture assay to compare exonic sequences of allotetraploid wheat accessions. Results: A sequence capture assay was designed for the targeted re-sequencing of 3.5 Mb exon regions that surveyed a total of 3,497 genes from allotetraploid wheat. These data were used to describe SNPs, copy number variation and homoeologous sequence divergence in coding regions. A procedure for variant discovery in the polyploid genome was developed and experimentally validated. About 1% and 24% of discovered SNPs were loss-of-function and non-synonymous mutations, respectively. Under-representation of replacement mutations was identified in several groups of genes involved in translation and metabolism. Gene duplications were predominant in a cultivated wheat accession, while more gene deletions than duplications were identified in wild wheat. Conclusions: We demonstrate that, even though the level of sequence similarity between targeted polyploid genomes and capture baits can bias enrichment efficiency, exon capture is a powerful approach for variant discovery in polyploids. Our results suggest that allopolyploid wheat can accumulate new variation in coding regions at a high rate. This process has the potential to broaden functional diversity and generate new phenotypic variation that eventually can play a critical role in the origin of new adaptations and important agronomic traits.Digital Object Identifier http://dx.doi.org/10.1186/gb-2011-12-9-r88
机译:背景:草种适应各种栖息地的能力归因于其基因组的动态特性,而这些基因组是由古代和近来的多倍体化形成的。为了更好地了解多倍体基因组功能相关区域的变异性质和程度,我们开发了一种序列捕获测定法,以比较同种二倍体小麦种质的外显子序列。结果:设计了一种序列捕获测定法,用于3.5 Mb外显子区域的靶向重测序,该序列调查了来自异源四倍体小麦的总共3,497个基因。这些数据用于描述编码区中的SNP,拷贝数变异和同源序列差异。开发了多倍体基因组中发现变异的方法,并进行了实验验证。发现的SNP分别约有1%和24%为功能丧失和非同义突变。在涉及翻译和代谢的几组基因中发现了替代突变的代表性不足。基因重复在栽培小麦中占主导地位,而在野生小麦中发现的基因缺失多于重复。结论:我们证明,即使靶向多倍体基因组和捕获诱饵之间的序列相似性水平可能会影响富集效率,外显子捕获还是多倍体中发现变异的有效方法。我们的结果表明,同种多倍体小麦可以在编码区高速率积累新的变异。该过程有可能扩大功能多样性并产生新的表型变异,最终在新的适应方法和重要的农艺性状的起源中发挥关键作用。数字对象标识符http://dx.doi.org/10.1186/gb-2011 -12-9-r88

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