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Electrophoretic Analysis of Biomarkers using Capillary Modification with Gold Nanoparticles Embedded in a Polycation and Boron Doped Diamond Electrode

机译:毛细管修饰金纳米粒子嵌入聚阳离子和掺硼金刚石电极中的毛细管修饰对生物标志物的电泳分析

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Field-amplified sample stacking using a fused silica capillary coated with gold nanoparticles (AuNPs) embedded in poly(diallyl dimethylammonium) chloride (PDDA) has been investigated for the electrophoretic separation of indoxyl sulfate, homovanillic acid (HVA), and vanillylmandelic acid (VMA). AuNPs (27 nm) exhibit ionic and hydrophobic interactions, as well as hydrogen bonding with the PDDA network to form a stable layer on the internal wall of the capillary. This approach reverses electro-osmotic flow allowing for fast migration of the analytes while retarding other endogenous compounds including ascorbic acid, uric acid, catecholamines, and indoleamines. Notably, the two closely related biomarkers of clinical significance, HVA and VMA, displayed differential interaction with PDDA-AuNPs which enabled the separation of this pair. The detection limit of the three analytes obtained by using a boron doped diamond electrode was approx75 nM, which was significantly below their normal physiological levels in biological fluids. This combined separation and detection scheme was applied to the direct analysis of these analytes and other interfering chemicals including uric and ascorbic acids in urine samples without off-line sample treatment or preconcentration.
机译:研究了使用包覆有金纳米颗粒(AuNPs)的熔融石英毛细管在现场放大的样品中堆叠的方法,该纳米颗粒嵌入了聚二烯丙基二甲基氯化铵(PDDA)中,用于电泳分离茚吲哚硫酸盐,高香草酸(HVA)和香草香草酸(VMA) )。 AuNPs(27 nm)表现出离子和疏水相互作用,以及与PDDA网络的氢键结合,从而在毛细管的内壁上形成稳定的层。这种方法可以逆转电渗流,使分析物快速迁移,同时阻止其他内源性化合物,包括抗坏血酸,尿酸,儿茶酚胺和吲哚胺。值得注意的是,具有临床意义的两个密切相关的生物标记物HVA和VMA与PDDA-AuNPs表现出不同的相互作用,从而可以分离该对。使用掺硼金刚石电极获得的三种分析物的检出限约为75 nM,大大低于其在生物液体中的正常生理水平。这种组合的分离和检测方案可直接用于尿液样品中的这些分析物和其他干扰化学物质(包括尿酸和抗坏血酸)的分析,而无需离线样品处理或预浓缩。

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