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Circle-to-circle amplification for precise and sensitive DNA analysis

机译:圆到圆扩增,可进行精确而敏感的DNA分析

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We present a tightly controlled process for strand-specific amplification of circularized DNA molecules. Tandem repeated complements of DNA circles are generated by rolling-circle replication, and converted to monomer circles of opposite polarity to that of the starting material. These circles are then subjected to one more round of rolling-circle replication and circularization, and the process can be further repeated. The method can be directed to produce single-stranded circular or linear monomers, or linear concatemers of the desired polarity. The reaction is not product inhibited, and can yield approximate to100-fold higher concentrations of monomer products than PCR. Each generation of the amplification process proceeds in a linear fashion, ensuring precise quantification. The procedure is suitable for parallel amplification of large numbers of DNA circles, because the few cycles and the robust reaction mechanism preserves the proportion of amplified molecules. We demonstrate the utility of the method for multiplexed genotyping of polymorphic loci and for quantitative DNA analysis. [References: 18]
机译:我们提出了严格控制的过程的环化DNA分子链特异性扩增。 DNA环的串联重复补体通过滚环复制生成,并转换为与起始材料极性相反的单体环。然后,对这些圆再进行一轮滚动圆复制和圆化处理,然后可以进一步重复该过程。该方法可用于生产所需极性的单链圆形或线性单体或线性连接体。该反应不受产物的抑制,并且可以产生比PCR高约100倍的单体产物浓度。每一代扩增过程均以线性方式进行,从而确保精确定量。该程序适用于大量DNA环的并行扩增,因为循环少,反应机理强,保留了扩增分子的比例。我们证明了该方法用于多态性基因座的基因分型和定量DNA分析的实用性。 [参考:18]

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