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Selective DNA amplification from complex genomes using universal double-sided adapters

机译:使用通用双面适配器从复杂基因组中选择性扩增DNA

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摘要

There is a rapidly developing need for new technologies to amplify millions of different targets from genomic DNA for high throughput genotyping and population gene-sequencing from diverse species. Here we describe a novel approach for the specific selection and amplification of genomic DNA fragments of interest that eliminates the need for costly and time consuming synthesis and testing of potentially millions of amplicon-specific primers. This technique relies upon Type IIs restriction enzyme digestion of genomic DNA and ligation of the fragments to double-sided adapters to form closed-circular DNA molecules. The novel use of double-sided adapters, assembled through the combinatorial use of two small universal sets of oligonucleotide building blocks, provides greater selection capacity by utilizing both sides of the adapter in a sequence-specific ligation event. As demonstrated, formation of circular structures results in protection of the desired molecules from nuclease treatment and enables a level of selectivity high enough to isolate single, or multiple, pre-defined fragments from the human genome when digested at over five million sites. Priming sites incorporated into the adapter allows the utilization of a common pair of primers for the amplification of any adapter-captured DNA fragment of interest.
机译:急需新技术以从基因组DNA扩增数百万个不同的靶标,以实现高通量的基因分型和来自不同物种的种群基因测序。在这里,我们描述了一种用于目标基因组DNA片段的特异性选择和扩增的新颖方法,它消除了对可能数百万个扩增子特异性引物进行昂贵且耗时的合成和测试的需求。该技术依赖于基因组DNA的II型限制性酶消化以及片段与双面衔接子的连接以形成封闭的环状DNA分子。通过结合使用两个小的通用的寡核苷酸构建基组组合组装而成的双面衔接子,通过在序列特异性连接事件中利用衔接子的两侧,提供了更大的选择能力。如证明的那样,形成圆形结构可保护所需分子免受核酸酶处理,并具有足够高的选择性,可在超过500万个位点消化时从人类基因组中分离出单个或多个预定片段。结合到衔接子中的引物位点允许利用通用的一对引物来扩增感兴趣的任何衔接子捕获的DNA片段。

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