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Integrated dielectrophoretic and surface plasmonic platform for million-fold improvement in the detection of fluorescent events

机译:集成的介电泳和表面等离激元平台可将荧光事件的检测提高百万倍

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摘要

We present an integrated dielectrophoretic (DEP) and surface plasmonic technique to quantify ∼1 pM of fluorescent molecules in low conductivity buffers. We have established a DEP force on target molecules to bring those molecules and place them on the nanometallic structures (hotspots) for quantification through surface plasmonic effects. Our results show that the DEP is capable of placing the fluorescent molecules on the hotspots, which are depicted as a significant reduction in the fluorescence lifetime of those molecules. To efficiently integrate the DEP and plasmonic effects, we have designed and utilized pearl-shaped interdigitated electrodes (PIDEs) in experiments. These electrodes generate 2–3 times higher DEP force than traditional interdigitated electrodes. Therefore, high-throughput assays can be developed. The nanometallic structures were strategically fabricated in the periphery of PIDEs for smooth integration of DEP and plasmonic detection. With the introduction of DEP, about 106-fold improvement was achieved over existing plasmonic-based detection. Therefore, this simple addition to the existing surface plasmonic-based detection will enable the disease related protein detection.
机译:我们提出了一种集成的介电电泳(DEP)和表面等离子体技术,以定量在低电导率缓冲液中的荧光分子〜1 pM。我们已经在目标分子上建立了DEP力,以将这些分子带入纳米金属结构(热点),以通过表面等离激元效应进行定量。我们的结果表明,DEP能够将荧光分子置于热点上,这被描述为这些分子的荧光寿命显着减少。为了有效地整合DEP和等离激元效应,我们在实验中设计并利用了珍珠形叉指电极(PIDE)。这些电极产生的DEP力是传统叉指电极的2-3倍。因此,可以开发高通量分析。在PIDE的外围策略性地制造了纳米金属结构,以实现DEP和等离子体检测的平滑整合。通过引入DEP,与现有的基于等离激元的检测相比,可实现约10 6 的改进。因此,对现有基于表面等离子的检测方法的简单补充将使与疾病相关的蛋白质检测成为可能。

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