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一种用于区分免疫比浊分析用商业人血清标准品的新型凝胶定量法。

A new specific quantitation-in-gel method differentiating commercial human serum standards intended for RID analyses.

作者信息

Wadsworth C

出版信息

Scand J Immunol. 1977;6(1-2):97-107. doi: 10.1111/j.1365-3083.1977.tb00325.x.

Abstract

A rapid, sensitive technique is described which measures small amounts of protein applied on agarose gel containing specific antibody. Alternating current through the gel reduces the influence of diffusion, and specific immunoprecipitate spots are formed. Their density after staining is proportional to applied protein. Quantitation of IgG and IgA in human serum standards was highly reproducible (P less than 0.001, Spearman coefficient of rank correlation test), and as little as about 35 ng Ig could be detected. Results are available within hours. Human sera and some purified preparations of 7S IgG and secretory IgA were grouped according to immuno-gel filtration findings. The group of samples containing fragments, aggregates, or unusually small amounts of monomeric IgG or IgA was also differentiated by specific immunoprecipitate spot (SIS) analysis from those mainly monomeric in character (Wilcoxon rank test, P less than 0.02). A World Health Organization reference serum (67/97) was used as standard. The study indicates that a human serum pool stored in aliquots at -20 degrees C is a good standard for quantitating serum IgG and IgA and that purified preparations are no better. It is suggested that the SIS assay could be advantageously applied to screening biologic fluids for unusual amounts or types of IgG and IgA.

摘要

本文描述了一种快速、灵敏的技术,该技术可测定施加在含有特异性抗体的琼脂糖凝胶上的少量蛋白质。通过凝胶的交流电可减少扩散的影响,并形成特异性免疫沉淀斑点。染色后其密度与施加的蛋白质成正比。人血清标准品中IgG和IgA的定量具有高度可重复性(P<0.001,Spearman等级相关检验系数),可检测到低至约35 ng的Ig。数小时内即可获得结果。根据免疫凝胶过滤结果,对人血清以及7S IgG和分泌型IgA的一些纯化制剂进行了分组。含有片段、聚集体或异常少量单体IgG或IgA的样本组,通过特异性免疫沉淀斑点(SIS)分析也与主要为单体性质的样本组区分开来(Wilcoxon秩检验,P<0.02)。使用世界卫生组织参考血清(67/97)作为标准品。该研究表明,在-20℃下分装储存的人血清库是定量血清IgG和IgA的良好标准品,纯化制剂并不更好。建议SIS测定法可有利地应用于筛选生物体液中异常量或类型的IgG和IgA。

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