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Neuronal Tau Protein Self-Assembly on Gold Surface: Electrochemical Impedance Spectroscopy and Cyclic Voltammetry Studies

机译:神经元Tau蛋白质在金表面上自组装:电化学阻抗光谱和循环伏安法研究

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Tau is a neuronal protein responsible for microtubule formation. It is also the pathological protein active in the Alzheimer's Disease (AD) pathway. When Tau begins to aggregate as a result of misfolding, the neuronal cells die due to the lack of microtubule formation and can take on prion-like properties. Therefore, detection of aggregated Tau can serve as a powerful tool in the early diagnosis of AD and dementia related diseases. As has been previously demonstrated, Tau 441 can be detected with an electrochemical immunoassay based on the electrochemical impedance spectroscopy (EIS) by using gold electrode. The EIS was also used to monitor interactions between Tau protein and Heparin. Herein, we describe use of EIS and cyclic voltammetry (CV) to monitor and detect self-assembly of Tau protein on gold electrode. After modifying the surface of the electrode with Tau, the aggregation of Tau was performed using Heparin, as an aggregation inducer. The EIS and CV were measured as a function of Tau or Heparin concentrations, and incubation time and temperature. The control experiments included, Tau-free surface, Heparin-free solution, buffer solution in order to minimize aggregation. The charge transfer resistance, R_(ct), was determined by fitting the experimental data to the equivalent circuit. The R_(ct) values for Tau-films on gold surface were compared prior and post aggregation. The R_(ct) values were highly dependent on the experimental conditions used and that the electrochemical methods are promising sensing platforms for detection of neurodegenerative biomarkers which undergo self-assembly and aggregation.
机译:Tau是一种负责微管形成的神经元蛋白。它也是阿尔茨海默病(AD)途径中活性的病理蛋白。当TAU由于误折叠而开始聚集时,神经元细胞因缺乏微管形成而导致的,并且可以采用朊病毒性质。因此,聚集的Tau的检测可以作为早期诊断和痴呆相关疾病的强大工具。如前所述,通过使用金电极,可以基于电化学阻抗光谱(EIS)用电化学免疫测定检测TAU 441。 EIS还用于监测Tau蛋白和肝素之间的相互作用。在此,我们描述了EIS和循环伏安法(CV)的用途来监测和检测金电极上TAU蛋白的自组装。在用TAU改变电极表面后,使用肝素进行TAU的聚集,作为聚集诱导剂。测量EIS和CV作为TAU或肝素浓度的函数,以及孵育时间和温度。控制实验包括,无土表面,无肝素溶液,缓冲溶液,以最小化聚集。通过将实验数据拟合到等效电路来确定电荷传递电阻R_(CT)。比较了金表面上的Tau-薄膜的R_(CT)值并在聚集后比较。 R_(CT)值高度依赖于所使用的实验条件,并且电化学方法是有前途的传感平台,用于检测经历自组装和聚集的神经变性生物标志物。

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