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Direct visualization of single-molecule translocations through synthetic nanopores comparable in size to a molecule

机译:通过合成纳米孔直接可视化单分子移位,其大小可与分子媲美

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摘要

A nanopore is the ultimate analytical tool. It can be used to detect DNA, RNA, oligonucleotides, and proteins with submolecular sensitivity. This extreme sensitivity is derived from the electric signal associated with the occlusion that develops during the translocation of the analyte across a membrane through a pore immersed in electrolyte. A larger occluded volume results in an improvement in the signal-to-noise ratio, and so the pore geometry should be made comparable to the size of the target molecule. However, the pore geometry also affects the electric field, the charge density, the electro-osmotic flow, the capture volume, and the response time. Seeking an optimal pore geometry, we tracked the molecular motion in three dimensions with high resolution, visualizing with confocal microscopy the fluorescence associated with DNA translocating through nanopores with diameters comparable to the double helix, while simultaneously measuring the pore current. Measurements reveal single molecules translocating across the membrane through the pore commensurate with the observation of a current blockade. To explain the motion of the molecule near the pore, finite-element simulations were employed that account for diffusion, electrophoresis, and the electro-osmotic flow. According to this analysis, detection using a nanopore comparable in diameter to the double helix represents a compromise between sensitivity, capture volume, the minimum detectable concentration, and response time.
机译:纳米孔是最终的分析工具。它可用于以亚分子敏感性检测DNA,RNA,寡核苷酸和蛋白质。这种极高的灵敏度源自与阻塞相关的电信号,该阻塞在分析物通过浸没在电解质中的孔跨膜移位的过程中形成。较大的阻塞体积会导致信噪比提高,因此应使孔的几何形状与目标分子的大小可比。但是,孔的几何形状也会影响电场,电荷密度,电渗流,捕获体积和响应时间。为了找到最佳的孔几何形状,我们以高分辨率跟踪了三维的分子运动,通过共聚焦显微镜观察了与DNA穿过直径可与双螺旋媲美的纳米孔相关的荧光,同时测量了孔电流。测量结果表明,与目前的封锁情况相称,单个分子通过整个孔穿过膜移位。为了解释分子在孔附近的运动,采用了有限元模拟,该模拟考虑了扩散,电泳和电渗流。根据该分析,使用直径可与双螺旋相当的纳米孔进行检测代表了灵敏度,捕获量,最小可检测浓度和响应时间之间的折衷。

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