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人体对钥孔戚血蓝蛋白的体内原发性IgM和IgG抗体反应的测量:免疫前IgM结合在抗原特异性酶联免疫吸附测定中的意义

Measurement of primary in vivo IgM- and IgG-antibody response to KLH in humans: implications of pre-immune IgM binding in antigen-specific ELISA.

作者信息

Korver K, Zeijlemaker W P, Schellekens P T, Vossen J M

出版信息

J Immunol Methods. 1984 Nov 30;74(2):241-51. doi: 10.1016/0022-1759(84)90291-6.

DOI:10.1016/0022-1759(84)90291-6
PMID:6501888
Abstract

The antigen Keyhole Limpet Hemocyanin (KLH) is often used to test the primary in vivo antibody response capacity in humans. However, measurement of IgM anti-KLH antibodies in ELISA is complicated by the presence of natural antibodies in human serum. This problem occurs particularly at low antibody levels, i.e. after immunization with low doses of antigen and, under these conditions, it was found to be impossible to assess a dose-response curve by immunizing a series of individuals with different suboptimal doses of KLH. This problem was circumvented by choosing conditions for minimal binding of pre-immune IgM and to correct for such binding. Although signal-to-background ratios were markedly improved by modifying the ELISA conditions, pre-immune IgM still showed binding to KLH due to interaction with polysaccharide determinants. This non-specific binding was correlated with the total IgM content of the samples. When anti-KLH activities before and after immunization were expressed relative to total serum IgM, a significant correction was achieved, resulting in a diminished inter-individual variability with respect to both pre-immune and post-immunization values. As with IgG-class antibodies to KLH, virtually no binding was observed in pre-immune sera. After expression of the anti-KLH response as a ratio between the post-immunization and pre-immunization titres, a dose of 50 micrograms was found to be sufficient to evoke a detectable IgG-antibody response in the 10 subjects tested. To elicit a positive IgM response, a minimal dose of 250 micrograms was required.

摘要

抗原钥孔血蓝蛋白(KLH)常用于检测人体体内的初次抗体应答能力。然而,在酶联免疫吸附测定(ELISA)中检测抗KLH IgM抗体时,人血清中天然抗体的存在会使检测变得复杂。这个问题在抗体水平较低时尤其明显,即在低剂量抗原免疫后,在这些条件下,发现通过用不同次优剂量的KLH免疫一系列个体来评估剂量反应曲线是不可能的。通过选择使免疫前IgM结合最小化的条件并校正这种结合来规避这个问题。尽管通过改变ELISA条件显著提高了信号与背景的比率,但免疫前IgM仍因与多糖决定簇相互作用而显示出与KLH的结合。这种非特异性结合与样品中的总IgM含量相关。当免疫前后的抗KLH活性相对于总血清IgM表达时,实现了显著的校正,导致免疫前和免疫后值的个体间变异性降低。与抗KLH的IgG类抗体一样,在免疫前血清中几乎未观察到结合。将抗KLH反应表示为免疫后和免疫前滴度之比后,发现50微克的剂量足以在10名受试对象中引发可检测到的IgG抗体反应。要引发阳性IgM反应,需要至少250微克的剂量。

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