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DNA-Modified Electrodes Fabricated Using Copper-Free Click Chemistry for Enhanced Protein Detection

机译:使用无铜点击化学法制造的DNA修饰电极,用于增强蛋白质检测

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摘要

A method of DNA monolayer formation has been developed using copper-free click chemistry that yields enhanced surface homogeneity and enables variation in the amount of DNA assembled; extremely low-density DNA monolayers, with as little as 5% of the monolayer being DNA, have been formed. These DNA-modified electrodes (DMEs) were characterized visually, with AFM, and electrochemically, and were found to facilitate DNA-mediated reduction of a distally bound redox probe. These low-density monolayers were found to be more homogeneous than traditional thiol-modified DNA monolayers, with greater helix accessibility through an increased surface area-to-volume ratio. Protein binding efficiency of the transcriptional activator TATA-binding protein (TBP) was also investigated on these surfaces and compared to that on DNA monolayers formed with standard thiol-modified DNA. Our low-density monolayers were found to be extremely sensitive to TBP binding, with a signal decrease in excess of 75% for 150 nM protein. This protein was detectable at 4 nM, on the order of its dissociation constant, with our low-density monolayers. The improved DNA helix accessibility and sensitivity of our low-density DNA monolayers to TBP binding reflects the general utility of this method of DNA monolayer formation for DNA-based electrochemical sensor development.
机译:已经开发出一种使用无铜咔嗒化学法形成DNA单层的方法,该方法可增强表面均匀性并能够改变组装的DNA数量。已经形成了极低密度的DNA单层,其中仅有5%的单层是DNA。这些DNA修饰的电极(DME)可以通过AFM进行目测和电化学表征,并且可以促进DNA介导的远端结合氧化还原探针的还原。发现这些低密度单层比传统的巯基修饰的DNA单层更均匀,通过增加的表面积体积比具有更高的螺旋可达性。还研究了在这些表面上转录激活因子TATA结合蛋白(TBP)的蛋白结合效率,并将其与标准硫醇修饰的DNA形成的DNA单层蛋白的结合效率进行了比较。我们的低密度单层膜对TBP结合极为敏感,对于150 nM蛋白,信号降低超过75%。在我们的低密度单分子层上,该蛋白在4 nM时可检测到其解离常数的顺序。低密度DNA单层对TBP结合的改进的DNA螺旋可及性和敏感性反映了这种DNA单层形成方法在基于DNA的电化学传感器开发中的一般用途。

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