适配体的创建及其在电阻式脉冲传感器中的应用

Mark Platt
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引用次数: 0

摘要

电阻式脉冲传感器(RPS)使得分子、蛋白质甚至纳米颗粒通过小通道时的传输机制得以表征。在这里,我们介绍了我们最近的技术进展,确定了潜在的POC分析的关键实验设计。第一个实验利用超顺磁珠,如果用适体修饰珠的表面,珠通过孔的频率(易位/分钟)可以与溶液中特定蛋白质的浓度有关。在这里,我们已经证明了成功地使用TRPS来观察两种蛋白质同时与其特定适配体的结合。然后,我们调整了测量策略,并证明了粒子的易位次数可以用来推断zeta电位,以测量DNA修饰粒子的zeta电位变化。通过测量DNA修饰纳米颗粒的易位次数与堆积密度、长度、结构和杂交时间的关系,我们观察到zeta电位的平均值和种群分布与DNA结构的关系存在明显差异。最后,我们提出了在可调孔平台上使用电阻脉冲或整流比率的分析之间的第一个比较。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Creating Aptamers and Their Use in Resisitive Pulse Sensors

Resistive pulse sensors, RPS, are allowing the transport mechanism of molecules, proteins and even nanoparticles to be characterized as they traverse small channels. Here we present our recent advancement of the technique identifying key experimental designs for potential POC assays. The first assay utilized superparamagnetic beads, if the surfaces of the beads are modified with an aptamer, the frequency of beads (translocations/minute) through the pore can be related to the concentration of specific proteins in the solution. Herein, we have demonstrated the successful use of TRPS to observe the binding of two proteins, to their specific aptamers simultaneously. We then adapt the measurement strategy and demonstrate that the translocation times of particles can be used to infer the zeta potential to measure the change in zeta potential of DNA modified particles. By measuring the translocation times of DNA modified nanoparticles as a function of packing density, length, structure, and hybridisation time, we observe a clear difference in zeta potential using both mean values, and population distributions as a function of the DNA structure. Finally we present the first comparison between assays that use resistive pulses or rectification ratios on a tunable pore platform.

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