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PCR amplification from single DNA molecules on magnetic beads in emulsion: application for high-throughput screening of transcription factor targets

机译:从乳液中磁珠上的单个DNA分子进行PCR扩增:用于转录因子靶标的高通量筛选

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摘要

We have developed a novel method of genetic library construction on magnetic microbeads based on solid-phase single-molecule PCR in a fine and robust water-phase compartment formed in water-in-oil (w/o) emulsions. In this method, critically diluted DNA fragments were distributed over the emulsion as templates, where beads crosslinked with multiple primers and other PCR components were encapsulated to form multiple reaction compartments. The delivered DNA was then amplified and covalently immobilized on the beads in parallel, within individual compartments, to construct a genetic library on beads (GLOBE), which was readily applicable to a genomewide global scanning of genetic elements recognized by a defined DNA-binding protein. We constructed a GLOBE of Paracoccus denitrificans and selected gene beads that were bound to the His-tagged transcription factor PhaR by flow cytometry. As a result of flow cytometry screening with an anti-His fluorescent antibody, the PhaR target fragments were enriched 1200-fold from this library with this system. Therefore, this system is a powerful tool for analyzing the transcription network on a genomewide scale.
机译:我们已经开发了一种基于固相单分子PCR的磁微珠上遗传库构建的新方法,该固相单分子PCR在油包水(w / o)乳液中形成的精细而坚固的水相隔室中。在这种方法中,将临界稀释的DNA片段作为模板分布在乳液中,其中与多个引物和其他PCR组分交联的珠子被封装起来以形成多个反应室。然后将所传递的DNA扩增并共价固定在各个小室内的小球上,以在小球上平行构建,以构建小球上的遗传文库(GLOBE),该文库可轻松应用于确定的DNA结合蛋白识别的遗传元件的全基因组全局扫描。我们构建了反硝化副球菌的GLOBE,并选择了通过流式细胞仪与His标记的转录因子PhaR结合的基因珠。用抗His荧光抗体进行流式细胞术筛选的结果是,使用该系统从该文库中富集了1200倍的PhaR目标片段。因此,该系统是用于在基因组范围内分析转录网络的强大工具。

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