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首页> 外文期刊>The Analyst: The Analytical Journal of the Royal Society of Chemistry: A Monthly International Publication Dealing with All Branches of Analytical Chemistry >Immunoassay using probe-labelling immunogold nanoparticles with silver staining enhancement via surface-enhanced Raman scattering
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Immunoassay using probe-labelling immunogold nanoparticles with silver staining enhancement via surface-enhanced Raman scattering

机译:使用探针标记的免疫金纳米颗粒通过表面增强拉曼散射增强银染的免疫分析

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This paper reports a novel immunoassay based on surface-enhanced Raman scattering (SERS) and immunogold labelling with silver staining enhancement. Immunoreactions between immunogold colloids modified by a Raman-active probe molecule (e.g., 4-mercaptobenzoic acid) and antigens, which were captured by antibody-assembled chips such as silicon or quartz, were detected via SERS signals of Raman-active probe molecule. All the self-assembled steps were subjected to the measurements of ultraviolet-visible (UV-vis) spectra to monitor the formation of a sandwich structure onto a substrate. The immunoassay was performed by a sandwich structure consisting of three layers. The first layer was composed of immobilized antibody molecules of mouse polyclonal antibody against Hepatitis B virus surface antigen (PAb) on a silicon or quartz substrate. The second layer was the complementary Hepatitis B virus surface antigen ( Antigen) molecules captured by PAb on the substrate. The third layer was composed of the probe-labelling immunogold nanoparticles, which were modified by mouse monoclonal antibody against Hepatitis B virus surface antigen (MAb) and 4-mercaptobenzoic acid (MBA) as the Raman-active probe on the surface of gold colloids. After silver staining enhancement, the antigen is identified by a SERS spectrum of MBA. A working curve of the intensity of a SERS signal at 1585 cm(-1) due to the nu(8a) aromatic ring vibration of MBA versus the concentration of analyte ( Antigen) was obtained and the non-optimized detection limit for the Hepatitis B virus surface antigen was found to be as low as 0.5 mug mL(-1). [References: 61]
机译:本文报道了一种基于表面增强拉曼散射(SERS)和具有银染增强作用的免疫金标记的新型免疫测定方法。通过拉曼活性探针分子的SERS信号检测被拉曼活性探针分子(例如4-巯基苯甲酸)修饰的免疫金胶体与抗原(被抗体组装的芯片如硅或石英捕获)之间的免疫反应。对所有自组装步骤进行紫外-可见(UV-vis)光谱的测量,以监测在基材上的夹心结构的形成。通过由三层组成的夹心结构进行免疫测定。第一层由固定在硅或石英基底上的抗乙型肝炎病毒表面抗原(PAb)的小鼠多克隆抗体的抗体分子组成。第二层是由PAb在底物上捕获的互补性乙型肝炎病毒表面抗原(Antigen)分子。第三层由探针标记的免疫金纳米粒子组成,该纳米粒子由抗乙型肝炎病毒表面抗原(MAb)和4-巯基苯甲酸(MBA)的小鼠单克隆抗体修饰,作为金胶体表面上的拉曼活性探针。银染增强后,通过MBA的SERS光谱鉴定抗原。获得了由于MBA的nu(8a)芳香环振动而在1585 cm(-1)处的SERS信号强度与分析物浓度(抗原)的关系曲线,并对乙型肝炎的非最佳检测限发现病毒表面抗原低至0.5杯mL(-1)。 [参考:61]

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