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Nanopore Single-Molecule Analysis of DNA Doxorubicin Interactions

机译:DNA阿霉素相互作用的纳米孔单分子分析

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Anticancer activity and toxicity of doxorubicin (Dox) are associated with its DNA intercalation. To understand the role in gene regulation and the drug mechanism, it is a challenge to detect the DNA-Dox interaction at the single-molecule level without the use of laborious, time-consuming labeling assays and an error-prone amplification method. Here, we utilized the simplest and cheapest, yet highly sensitive, single-molecule nanopore technology to investigate the DNA-Dox interaction and explore in situ the intercalative reaction kinetics. Distinctive electronic signal patterns between DNA and the DNA-Dox complex allow protein nanopore to readily detect the changes in structure and function of DNA. After Dox insertion, nanopore unzipping time of DNA was elevated 10-fold while the blocking current decreased, demonstrating the higher affinity of the DNA-Dox complex (formation constant Kf = 3.09 x 10 (5) M-1). Continuous rapid nanopore detection in real time displayed that Dox intercalation in DNA is a two-state dynamic process: fast binding and slow conformational adaption. The nanopore platform provides a powerful tool for studying small molecule-biomacromolecule interactions and paves the way for novel applications aimed at drug screening and functional analysis.
机译:阿霉素(Dox)的抗癌活性和毒性与其DNA嵌入有关。要了解基因调节和药物作用机制中的作用,挑战是在不使用费力且费时的标记测定法和易于出错的扩增方法的情况下检测单分子水平的DNA-Dox相互作用。在这里,我们利用最简单,最便宜,但最灵敏的单分子纳米孔技术来研究DNA-Dox相互作用并原位研究嵌入反应动力学。 DNA与DNA-Dox复合物之间独特的电子信号模式使蛋白质纳米孔可以轻松检测DNA结构和功能的变化。插入Dox后,DNA的纳米孔解压缩时间增加了10倍,而阻断电流降低,表明DNA-Dox复合物具有更高的亲和力(形成常数Kf = 3.09 x 10(5)M-1)。实时连续快速的纳米孔检测表明,DNA中的Dox嵌入是两个状态的动态过程:快速结合和缓慢构象适应。纳米孔平台为研究小分子与生物大分子的相互作用提供了强大的工具,并为针对药物筛选和功能分析的新应用铺平了道路。

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