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Probe accessibility effects on the performance of electrochemical biosensors employing DNA monolayers

机译:探针可及性对采用DNA单层的电化学生物传感器性能的影响

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Surface-confined DNA probes are increasingly used as recognition elements (or presentation scaffolds) for detection of proteins, enzymes, and other macromolecules. Here we demonstrate that the density of the DNA probe monolayer on the gold electrode is a crucial determinant of the final signalling of such devices. We do so using redox modified single-stranded and double-stranded DNA probes attached to the surface of a gold electrode and measuring the rate of digestion in the presence of a non-specific nuclease enzyme. We demonstrate that accessibility of DNA probes for binding to their macromolecular target is, as expected, improved at lower probe densities. However, with double-stranded DNA probes, even at the lowest densities investigated, a significant fraction of the immobilized probe is inaccessible to nuclease digestion. These results stress the importance of the accessibility issue and of probe density effects when DNA-based sensors are used for detection of macromolecular targets.
机译:表面受限的DNA探针越来越多地用作识别元素(或呈递支架),用于检测蛋白质,酶和其他大分子。在这里,我们证明了金电极上DNA探针单层的密度是此类设备最终信号的关键决定因素。我们使用附着在金电极表面的氧化还原修饰的单链和双链DNA探针,并在存在非特异性核酸酶的情况下测量消化速率。我们证明,DNA探针与其大分子靶标结合的可及性如预期的那样,在较低的探针密度下得到了改善。但是,使用双链DNA探针,即使以最低的密度进行研究,核酸酶的消化也很难达到固定化探针的很大一部分。这些结果强调了基于DNA的传感器用于检测大分子靶标时,可及性问题和探针密度效应的重要性。

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