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Noncovalent Antibody Immobilization on Porous Silicon Combined with Miniaturized Solid-Phase Extraction (SPE) for Array Based ImmunoMALDI Assays

机译:非共价抗体固定在多孔硅上结合微型固相萃取(SPE)进行基于阵列的ImmunoMALDI分析

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摘要

This paper presents a new strategy to combine the power of antibody based capturing of target species in complex samples with the benefits of microfluidic reverse phase sample preparation on an integrated sample enrichment target (RP-ISET) and the analysis speed of MALDI MS. The immunoaffinity step is performed on an in-house developed 3D-structured high surface area porous silicon (PSi) matrix, which allows efficient antibody immobilization by surface adsorption without any coupling agents in 30-60 min. The hydrophilic nature of the porous silicon surface at the molecular level displays a low adsorption of background peptides when exposed to complex digests or plasma samples, improving the conditions for the antigen specific extraction and subsequent readout. At the same time, the hydrophobic behavior, due to the nanostructured surface, of the PSi material facilitates liquid confinement during the assay. Using a footprint conforming to the standard for 384 well microplates, direct adaption of the protocol into standard sample handling robots is possible. The performance of the proposed immunoaffinity PSi-ISET immunoMALDI (iMALDI) assay was evaluated by specific detection of angiotensin I at a 10 femtomol level in diluted plasma samples (10 (mu)L, 1 nM).
机译:本文提出了一种新策略,该策略将基于抗体的复杂样本中目标物种的捕获功能与基于整体样本富集目标(RP-ISET)的微流控反相样本制备的优势以及MALDI MS的分析速度相结合。免疫亲和步骤在内部开发的3D结构的高表面积多孔硅(PSi)基质上进行,可在30-60分钟内通过表面吸附有效地固定抗体,而无需任何偶联剂。当暴露于复杂的消化液或血浆样品中时,多孔硅表面在分子水平上的亲水性表现出背景肽的低吸附性,从而改善了抗原特异性提取和后续读数的条件。同时,由于纳米结构的表面,PSi材料的疏水行为促进了测定期间的液体限制。使用符合384孔微孔板标准的占地面积,可以将方案直接适配到标准样品处理机器人中。通过特异性检测稀释血浆样品(10μL,1 nM)中浓度为10飞摩尔的血管紧张素I,评估了拟议的免疫亲和PSi-ISET免疫MALDI(iMALDI)分析的性能。

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