Kenny G E, Dunsmoor C L
J Clin Microbiol. 1983 Apr;17(4):655-65. doi: 10.1128/jcm.17.4.655-665.1983.
Competition between proteins and other macromolecules for adsorption sites on plastic was studied with the enzyme-linked immunosorbent assay (ELISA) to determine effects of the use of antigenic mixtures or extracts of organisms on assays of antibodies and antigens by ELISA. A comparison of a number of different polystyrene microplates with bovine albumin and human immunoglobulin G (IgG) as antigens showed two major classes of plates; those which adsorbed albumin poorly and those which adsorbed albumin well. IgG adsorbed well on all plates, but plates which adsorbed albumin best also gave significant background levels of nonspecific binding of conjugate. When mixtures of IgG and bovine serum albumin were used as coating antigens, significant competition was observed; the component present at 1% or less in the mixture was essentially undetectable unless excessive amounts of conjugate were used. The important factor was the ratio of competitor to antigen, not the absolute amount. Other proteins (ovalbumin, rabbit albumin, human albumin, and gelatin) were equally effective competitors for adsorption sites on plastic. Nonionic detergents (Tween 20, and Triton X-100) were strong competitors even at 10:1 competitor-to-antigen ratios. In antigen capture assays, normal serum components blocked attachment of antigen-specific IgG, but this competition could be lessened to a degree by the use of strongly binding polystyrene plates. In indirect ELISA for measurement of serum antibody, the use of antigenic mixtures gave significantly lower antibody titers when the desired antigen was less than 1% of the total protein coated. Therefore, the use of mixed or crude antigens in ELISA presents significant problems concerning the sensitivity and specificity of tests.
采用酶联免疫吸附测定法(ELISA)研究了蛋白质和其他大分子在塑料表面吸附位点上的竞争情况,以确定使用生物抗原混合物或提取物对ELISA检测抗体和抗原的影响。以牛血清白蛋白和人免疫球蛋白G(IgG)作为抗原,对多种不同的聚苯乙烯微孔板进行比较,结果显示有两大类微孔板:一类对白蛋白吸附较差,另一类对白蛋白吸附良好。IgG在所有微孔板上都吸附良好,但对白蛋白吸附最佳的微孔板也会出现显著的结合物非特异性结合背景水平。当使用IgG和牛血清白蛋白的混合物作为包被抗原时,观察到显著的竞争现象;混合物中含量为1%或更低的成分基本上无法检测到,除非使用过量的结合物。重要的因素是竞争者与抗原的比例,而非绝对量。其他蛋白质(卵清蛋白、兔血清白蛋白、人血清白蛋白和明胶)对塑料表面的吸附位点同样具有有效的竞争作用。非离子型去污剂(吐温20和曲拉通X-100)即使在竞争者与抗原比例为10:1时也是强竞争者。在抗原捕获测定中,正常血清成分会阻断抗原特异性IgG的附着,但使用强结合聚苯乙烯微孔板可在一定程度上减轻这种竞争。在用于检测血清抗体的间接ELISA中,当所需抗原占包被总蛋白的比例小于1%时,使用抗原混合物会使抗体滴度显著降低。因此,在ELISA中使用混合或粗制抗原会给检测的灵敏度和特异性带来重大问题。