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[使用生物素-链霉亲和素系统提高免疫分析参数]

[The use of biotin-streptavidin systems for enhancing the parameters of immunometric analysis].

作者信息

Lepesheva G I, Martsev S P

出版信息

Zh Mikrobiol Epidemiol Immunobiol. 1990 Oct(10):121-5.

PMID:2075757
Abstract

The possibility of improving analytical parameters of the immunometric assay with the use of biotinylated antibodies and biotin-streptavidin complexes in comparison with the commonly known approach of direct antibody modification with 125I has been studied. Experiments have been carried out with the use of low-affinity antibodies (Kass approximately 10(9) M-1) to ferritin. The signal-to-noise ratio in the immunometric increases 2.3 times when streptavidin labeled with horse-radish peroxidase is used and 4.3 times when the preformed streptavidin + biotin-peroxidase complex is used in comparison with assay systems based on 125I-labeled antibodies. The improvement of assay parameters of immunochemical systems by means of biotin-streptavidin complexes has been found to permit the use of low-affinity antibodies as assay reagents, thus ensuring analytical parameters attaining or close to those of immunoradiometric assay systems based on high-affinity 125I-labeled antibodies (Kass approximately 10(10) M-1). As shown in this study, the following factors ensure the signal enhancement in biotin-streptoavidin systems: (a) the biotin modification of several lysin residues per IgG molecule, the optimum extent of modification being 3-4 residues per molecule; (b) mild procedure for biotinylation. In contrast to oxidative iodination, the modification of NH2 groups with biotin esters does not significantly affect their antigen-binding properties.

摘要

与用¹²⁵I直接修饰抗体的常用方法相比,研究了使用生物素化抗体和生物素-链霉亲和素复合物改善免疫测定分析参数的可能性。使用对铁蛋白亲和力低的抗体(亲和常数Kass约为10⁹M⁻¹)进行了实验。与基于¹²⁵I标记抗体的分析系统相比,当使用辣根过氧化物酶标记的链霉亲和素时,免疫测定中的信噪比提高了2.3倍,当使用预先形成的链霉亲和素+生物素-过氧化物酶复合物时,信噪比提高了4.3倍。已发现通过生物素-链霉亲和素复合物改善免疫化学系统的分析参数可以允许使用低亲和力抗体作为分析试剂,从而确保分析参数达到或接近基于高亲和力¹²⁵I标记抗体(亲和常数Kass约为10¹⁰M⁻¹)的免疫放射分析系统的参数。如本研究所示,以下因素可确保生物素-链霉亲和素系统中的信号增强:(a) 每个IgG分子对几个赖氨酸残基进行生物素修饰,最佳修饰程度为每个分子3-4个残基;(b) 生物素化的温和程序。与氧化碘化不同,用生物素酯修饰NH₂基团不会显著影响其抗原结合特性。

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