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[使用辣根过氧化物酶对人免疫球蛋白G进行均相免疫酶分析]

[Homogeneous immunoenzyme analysis of human immunoglobulin G using horseradish peroxidase].

作者信息

Savenkova M N

出版信息

Prikl Biokhim Mikrobiol. 1991 Mar-Apr;27(2):265-73.

PMID:2062824
Abstract

The author studied the steady-state kinetics of cooxidation of 4-aminoantipyrine (AAP) with phenol and its derivatives--alpha-naphthol, o- and m-acetylaminophenols--by horseradish peroxidase and its conjugate with human immunoglobulins IgG (HRP-IgG). When phenol and AAP were used as peroxidase substrates, anti-human IgG antibodies stimulated the HPR-IgG enzyme activity in the presence of excess H2O2. A homogeneous enzyme immunoassay of human IgG was developed on the basis of this stimulating effect. The kinetics of the interactions between immunological reagents was studied. In the presence of 3% polyethylene glycol 6000, a complete antibody-antigen interaction proceeds at 37 degrees for 15-20 min. The sensitivity of the enzyme immunoassay is 350 ng/ml IgG, and the dynamic detection range is 0.35-15.0 mg/ml.

摘要

作者研究了辣根过氧化物酶及其与人免疫球蛋白IgG的缀合物(HRP-IgG)催化4-氨基安替比林(AAP)与苯酚及其衍生物——α-萘酚、邻乙酰氨基酚和间乙酰氨基酚共氧化的稳态动力学。当苯酚和AAP用作过氧化物酶底物时,在过量过氧化氢存在下,抗人IgG抗体刺激HPR-IgG酶活性。基于这种刺激作用,开发了一种人IgG的均相酶免疫测定法。研究了免疫试剂之间相互作用的动力学。在3%聚乙二醇6000存在下,抗体-抗原完全相互作用在37℃下进行15-20分钟。该酶免疫测定法的灵敏度为350 ng/ml IgG,动态检测范围为0.35-15.0 mg/ml。

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