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Proximity hybridization-mediated isothermal exponential amplification for ultrasensitive electrochemical protein detection

机译:邻近杂交介导的等温指数扩增用于超灵敏的电化学蛋白质检测

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摘要

In this study, we fabricated a novel electrochemical biosensing platform on the basis of target-triggered proximity hybridization-mediated isothermal exponential amplification reaction (EXPAR) for ultrasensitive protein analysis. Through rational design, the aptamers for protein recognition were integrated within two DNA probes. Via proximity hybridization principle, the affinity protein-binding event was converted into DNA assembly process. The recognition of protein by aptamers can trigger the strand displacement through the increase of the local concentrations of the involved probes. As a consequence, the output DNA was displaced, which can hybridize with the duplex probes immobilized on the electrode surface subsequently, leading to the initiation of the EXPAR as well as the cleavage of duplex probes. Each cleavage will release the gold nanoparticles (AuNPs) binding sequence. With the modification of G-quadruplex sequence, electrochemical signals were yielded by the AuNPs through oxidizing 3,3′,5,5′-tetramethylbenzidine in the presence of H2O2. The study we proposed exhibited high sensitivity toward platelet-derived growth factor BB (PDGF-BB) with the detection limit of 52 fM. And, this method also showed great selectivity among the PDGF isoforms and performed well in spiked human serum samples.
机译:在这项研究中,我们基于目标触发的邻近杂交介导的等温指数扩增反应(EXPAR)制备了新型电化学生物传感平台,用于超灵敏蛋白质分析。通过合理的设计,用于蛋白质识别的适体被整合到两个DNA探针中。通过邻近杂交原理,亲和蛋白结合事件被转化为DNA组装过程。适体对蛋白质的识别可通过增加所涉及探针的局部浓度来触发链置换。结果,输出的DNA被置换,其随后可与固定在电极表面上的双链探针杂交,导致EXPAR的起始以及双链探针的裂解。每次切割将释放金纳米颗粒(AuNPs)结合序列。通过修饰G-四链体序列,AuNPs在H2O2存在下通过氧化3,3',5,5'-四甲基联苯胺产生电化学信号。我们提出的研究显示对血小板衍生的生长因子BB(PDGF-BB)的高灵敏度,检测极限为52 fM。而且,该方法还显示出PDGF亚型之间的巨大选择性,并且在加标的人血清样品中表现良好。

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