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用于开发无标记抗凝血酶适体传感器的改良金平台的特性描述。

Characterization of a modified gold platform for the development of a label-free anti-thrombin aptasensor.

机构信息

Instituto de Investigaciones en Físico Química de Córdoba (INFIQC) CONICET-UNC, Departamento de Físico Química, Facultad de Ciencias Químicas, Universidad Nacional de Córdoba, Ciudad Universitaria, 5000 Córdoba, Argentina.

出版信息

Biosens Bioelectron. 2013 Mar 15;41:424-9. doi: 10.1016/j.bios.2012.08.061. Epub 2012 Sep 8.

Abstract

This work reports the characterization of a modified gold surface as a platform for the development of a label free aptasensor for thrombin detection. The biorecognition platform was obtained by the self-assembly of 4-mercaptobenzoic acid onto a gold surface, covalent attachment of streptavidin and further immobilization of the biotinylated anti-thrombin aptamer. The biosensing platform was characterized by cyclic voltammetry, electrochemical impedance spectroscopy, surface plasmon resonance (SPR) and quartz crystal microbalance with dissipation monitoring. The biorecognition event aptamer-thrombin was detected from changes in the SPR angle produced as a consequence of the molecular interaction between the aptasensor and the target protein. The biosensing platform demonstrated to be highly selective for human thrombin even in the presence of large excess of bovine thrombin, bovine serum albumin, cytochrome C, lysozyme and myoglobin. The relationship between the changes in the SPR angle and thrombin concentration was linear up to 0.19 μmol L(-1) (R(2)=0.992) while the detection limit was of 12.0 nmol L(-1) (240 fmol in the sample). This new sensing approach represents an interesting and promising alternative for the SPR-based quantification of thrombin.

摘要

本工作报道了一种改良金表面的特性,将其作为一种无标记适体传感器用于凝血酶检测的平台。该生物识别平台是通过 4-巯基苯甲酸自组装到金表面上,然后共价连接链霉亲和素,进一步固定生物素化抗凝血酶适体而获得的。通过循环伏安法、电化学阻抗谱、表面等离子体共振(SPR)和石英晶体微天平耗散监测对生物传感平台进行了表征。生物识别事件适体-凝血酶通过适体传感器与目标蛋白之间的分子相互作用产生的 SPR 角的变化来检测。该生物传感平台对人凝血酶具有高度选择性,即使在存在大量牛凝血酶、牛血清白蛋白、细胞色素 C、溶菌酶和肌红蛋白的情况下也是如此。SPR 角的变化与凝血酶浓度之间的关系在 0.19 μmol L(-1) 范围内呈线性关系(R(2)=0.992),而检测限为 12.0 nmol L(-1)(样品中为 240 fmol)。这种新的传感方法为基于 SPR 的凝血酶定量提供了一种有趣且有前途的替代方法。

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