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Single-molecule kinetics and super-resolution microscopy by fluorescence imaging of transient binding on DNA origami

机译:DNA折纸上瞬时结合的荧光成像的单分子动力学和超分辨率显微镜

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摘要

DNA origami is a powerful method for the programmable assembly of nanoscale molecular structures. For applications of these structures as functional biomaterials, the study of reaction kinetics and dynamic processes in real time and with high spatial resolution becomes increasingly important. We present a single-molecule assay for the study of binding and unbinding kinetics on DNA origami. We find that the kinetics of hybridization to single-stranded extensions on DNA origami is similar to isolated substrate-immobilized DNA with a slight position dependence on the origami. On the basis of the knowledge of the kinetics, we exploit reversible specific binding of labeled oligonucleotides to DNA nanostructures for PAINT (points accumulation for imaging in nanoscale topography) imaging with <30 nm resolution. The method is demonstrated for flat monomeric DNA structures as well as multimeric, ribbon-like DNA structures.
机译:DNA折纸是用于纳米分子结构可编程组装的有力方法。对于将这些结构用作功能性生物材料,实时且具有高空间分辨率的反应动力学和动力学过程的研究变得越来越重要。我们提出了一种单分子测定法,用于研究对DNA折纸的结合和解离动力学。我们发现,在DNA折纸上与单链延伸杂交的动力学与分离的底物固定的DNA相似,对折纸的位置稍有依赖性。在动力学知识的基础上,我们利用标记的寡核苷酸与DNA纳米结构的可逆特异性结合,以小于30 nm的分辨率进行PAINT(纳米级地形成像中的点积聚)成像。该方法可用于平坦的单体DNA结构以及多聚体,带状DNA结构。

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