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一种基于剪切增强的 CNT 组装纳米传感器平台,用于超灵敏和选择性蛋白质检测。

A shear-enhanced CNT-assembly nanosensor platform for ultra-sensitive and selective protein detection.

机构信息

Department of Chemical and Biomolecular Engineering, University of Notre Dame, 321 Stinson Remick, Notre Dame, IN 46556, United States.

出版信息

Biosens Bioelectron. 2017 Nov 15;97:143-149. doi: 10.1016/j.bios.2017.05.053. Epub 2017 May 31.

DOI:10.1016/j.bios.2017.05.053
PMID:28587929
Abstract

Detection and quantification of low-concentration proteins in heterogeneous media are generally plagued by two distinct obstacles: lack of sensitivity due to high dissociation equilibrium constant K and non-specificity due to an abundance of non-targets with similar K. Herein, we report a nanoscale protein-sensing platform with a non-equilibrium on-off switch that employs dielectrophoretic and hydrodynamic shear forces to overcome these thermodynamic limitations with irreversible kinetics. The detection sensitivity is achieved with complete association of the antibody-antigen-antibody (Ab-Ag-Ab) complex by precisely and rapidly assembling carbon nanotubes (CNT) across two parallel electrodes via sequential DC electrophoresis and AC dielectrophoresis (DEP), and with single-CNT electron tunneling conductance. The high selectivity is achieved with a critical hydrodynamic shear rate between the activated dissociation shear rates of target and non-target linkers of the aligned CNTs. We are able to reach detection limits of 100 attomolar (aM) and 10 femtomolar (fM) in pure samples for two ELISA assays with low and high dissociation constant: biotin/streptavidin (10 fM) and HER2/HER2 antibody (0.44 ± 0.07nM), respectively. For both models, irreversible capture and shearing allow us to tune the dynamic range up to 5 decades by increasing the CNT numbers. We also demonstrate in spiked serum sample high selectivity towards target HER2 proteins against non-target HER2 isoform of a similar K. The detection limit for HER2 in serum is lower than 100fM.

摘要

在不均匀介质中检测和定量低浓度蛋白质通常受到两个明显障碍的困扰

由于解离平衡常数 K 较高而导致灵敏度不足,以及由于具有相似 K 的大量非靶标存在而导致非特异性。在此,我们报告了一种具有非平衡开-关的纳米级蛋白质传感平台,该平台利用介电泳和流体动力剪切力来克服这些热力学限制,具有不可逆动力学。通过顺序直流电泳和交流介电泳(DEP)以及单根碳纳米管(CNT)的电子隧道传导,精确且快速地将 CNT 跨两个平行电极组装在一起,使抗体-抗原-抗体(Ab-Ag-Ab)复合物完全结合,从而实现检测灵敏度。通过激活的目标和非目标 CNT 对准的接头的解离剪切速率之间的临界流体动力剪切速率,实现了高选择性。我们能够在两种 ELISA 测定中达到 100 飞摩尔(aM)和 10 皮摩尔(fM)的检测极限,对于具有低和高解离常数的两个模型:生物素/链霉亲和素(10 fM)和 HER2/HER2 抗体(0.44 ± 0.07nM)。对于这两种模型,不可逆的捕获和剪切允许我们通过增加 CNT 的数量将动态范围调节高达 5 个数量级。我们还在加标血清样本中证明了针对具有相似 K 的非靶标 HER2 同工型的高选择性针对靶标 HER2 蛋白。血清中 HER2 的检测限低于 100fM。

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