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Feasibility studies of simultaneous multianalyte amperometric immunoassay based on spatial resolution.

机译:基于空间分辨率的同时多分析物安培免疫测定的可行性研究。

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摘要

A multianalyte immunoassay concept based on the geometric separation of different analyte-specific antibodies has been demonstrated. The assay and amperometric detection are done in a cell with two working electrodes controlled at the same potential, and the amperometric signal at each electrode is monitored. The distance between any two adjacent electrodes in this prototype is 2.5 mm, and during the course of amperometric measurement, the product formed at one electrode does not reach the other working electrode within 20 min after the addition of enzyme substrate. Thus, the method relies on the spatial resolution between the different antibodies being such that measurements are taken before cross-interference due to diffusion can occur. Identical enzyme labels (alkaline phosphatase, ALP) and substrates (p-aminophenyl phosphate, PAPP) are used for all analytes. Alkaline phosphatase-conjugated rat anti-mouse IgG was immobilized by passive adsorption. Our studies showed that this concept is feasible and can be applied to the simultaneous measurement of multiple analytes.
机译:已经证明了基于不同分析物特异性抗体的几何分离的多分析物免疫测定概念。该测定法和安培检测是在一个单元中完成的,两个工作电极被控制在相同的电势下,并监控每个电极上的安培信号。在该原型中,任何两个相邻电极之间的距离为2.5 mm,在安培测量过程中,在一个酶上形成的产物在添加酶底物后20分钟内不会到达另一个工作电极。因此,该方法依赖于不同抗体之间的空间分辨率,使得在可以发生由于扩散引起的交叉干扰之前进行测量。相同的酶标记物(碱性磷酸酶,ALP)和底物(对氨基苯基磷酸酯,PAPP)用于所有分析物。碱性磷酸酶偶联的大鼠抗小鼠IgG通过被动吸附固定化。我们的研究表明,该概念是可行的,可以应用于同时测量多种分析物。

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