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作为一种均相免疫测定法的磁性纳米颗粒磁光弛豫的测定。

Determination of the magneto-optical relaxation of magnetic nanoparticles as a homogeneous immunoassay.

作者信息

Aurich Konstanze, Nagel Stefan, Glöckl Gunnar, Weitschies Werner

机构信息

Institute of Pharmacy, Department of Biopharmaceutics and Pharmaceutical Technology, University of Greifswald, Friedrich-Ludwig-Jahn-Strasse 17, 17487 Greifswald, Germany.

出版信息

Anal Chem. 2007 Jan 15;79(2):580-6. doi: 10.1021/ac060491r.

Abstract

The interaction between human eotaxin (hEotaxin) and its polyclonal antibody anti-human eotaxin (anti-hEotaxin) was investigated by means of a novel liquid-phase immunoassay using the magneto-optical relaxation of ferrofluids. The binding quality as well as kinetic properties of the binding partners was determined using specifically binding magnetic probes. For this purpose, magnetic nanoparticles (MNP; DDM128N, Meito Sangyo, Japan) were initially functionalized with streptavidin. The biotin-nylated antibody was conjugated with streptavidin-MNP applying the streptavidin-biotin binding system. Binding reactions were detected by measuring the relaxation of the optical birefringence signal occurring when a pulsed magnetic field is applied to the ferrofluid. The addition of hEotaxin to anti-hEotaxin conjugated MNP in different amounts yielded an enlargement of the mean relaxation time due to the formation of MNP aggregates. In order to express the observed increase of the particles' effective diameter in terms of elementary kinetic processes between antigen and antibody, a kinetic model was introduced. Here, the binding reactions are described by a process of stepwise polymerization. The obtained results were compared with data received from surface plasmon resonance biosensor analysis, a standard tool for biomolecular interaction analysis.

摘要

采用一种利用铁磁流体磁光弛豫的新型液相免疫测定法,研究了人嗜酸性粒细胞趋化因子(hEotaxin)与其多克隆抗体抗人嗜酸性粒细胞趋化因子(抗hEotaxin)之间的相互作用。使用特异性结合磁探针测定结合伙伴的结合质量和动力学性质。为此,首先用链霉亲和素对磁性纳米颗粒(MNP;DDM128N,日本名东产业)进行功能化。应用链霉亲和素-生物素结合系统,将生物素化抗体与链霉亲和素-MNP偶联。通过测量向铁磁流体施加脉冲磁场时出现的光学双折射信号的弛豫来检测结合反应。向不同量的抗hEotaxin偶联MNP中添加hEotaxin,由于MNP聚集体的形成,平均弛豫时间延长。为了根据抗原与抗体之间的基本动力学过程来表达观察到的颗粒有效直径的增加,引入了一个动力学模型。在此,结合反应通过逐步聚合过程来描述。将获得的结果与从表面等离子体共振生物传感器分析(一种生物分子相互作用分析的标准工具)获得的数据进行比较。

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