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Quantitative Evaluation of Sensitivity and Selectivity of Multiplex NanoSPR Biosensor Assays

机译:多重NanoSPR生物传感器检测方法灵敏度和选择性的定量评估

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摘要

A new functionalization procedure was developed to replace cyltrimethylammoniumbromide coating on gold nanorods (GNRs) fabricated through seed-mediated growth with chemically active alkanethiols; antibodies were then attached to the GNRs to yield gold nanorod molecular probes (GNrMPs). The functionalization procedure was shown to minimize nonspecific binding. Multiplex sensing was demonstrated for three targets (goat anti-human IgG, goat anti-rabbit IgG, and goat anti-mouse IgG) through the distinct response of the plasmon spectra of GNrMPs to binding events. Quantification of the plasmonic binding events and estimation of ligand binding kinetics tethered to these nanoscale structures was also demonstrated through a mathematical approach. Evaluation of the experimental and theoretical data yields an affinity constant Ka = 1.34 × 107 M−1, which was in agreement with the IgG-antiIgG binding affinity reported in the literature. The GNrMP sensors were found to be highly specific and sensitive with the dynamic response in the range between 10−9 M and 10−6 M. The limit of detection of GNrMPs was found to be in the low nanomolar range, and is a function of the binding affinity: for a higher probe-target affinity pair, the limit of detection can be expected to reach femto molar levels. This technique can play a key role in developing tunable sensors for sensitive and precise monitoring of biological interactions.
机译:开发了一种新的功能化程序,以用化学活性的链烷硫醇代替通过种子介导的生长制得的金纳米棒(GNR)上的三甲基溴化铵。然后将抗体连接到GNR,以产生金纳米棒分子探针(GNrMP)。显示功能化程序使非特异性结合最小化。通过GNrMP的等离激元光谱对结合事件的独特响应,证明了三个靶标(山羊抗人IgG,山羊抗兔IgG和山羊抗小鼠IgG)的多重传感。还通过数学方法证明了等离激元结合事件的定量和束缚于这些纳米级结构的配体结合动力学的估计。对实验和理论数据的评估得出亲和常数Ka = 1.34×107 M-1,这与文献中报道的IgG-抗IgG结合亲和力一致。发现GNrMP传感器具有高度特异性和灵敏性,其动态响应范围在10-9 M和10-6 M之间。发现GNrMPs的检出限在低纳摩尔范围内,并且是结合亲和力:对于更高的探针-靶标亲和力对,检测极限有望达到毫微微摩尔水平。这项技术在开发可调节传感器以灵敏且精确地监测生物相互作用方面可以发挥关键作用。

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