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采用非竞争性免疫比浊法测定血清中的孕酮。

The measurement of progesterone in serum by a non-competitive idiometric assay.

作者信息

Barnard G, Osher J, Lichter S, Gayer B, De Boever J, Limor R, Ayalon D, Kohen F

机构信息

Department of Hormone Research, Weizmann Institute of Science, Rehovot, Israel.

出版信息

Steroids. 1995 Dec;60(12):824-9. doi: 10.1016/0039-128x(95)00144-f.

Abstract

A novel non-competitive idiometric time-resolved fluoroimmunoassay for the determination of serum progesterone was developed, based on the use of two types of anti-idiotypic antibody that recognize different epitopes within the hypervariable region of the primary antiprogesterone antibody. The first anti-idiotype, the betatype, competes with progesterone for an epitope of the primary antiprogesterone antibody at the binding site. The second anti-idiotype, the alphatype, binds to the antiprogesterone antibody in the presence of progesterone, but does not bind to the betatype antiprogesterone complex due to epitope proximity. In the present configuration, the biotinylated alphatype was captured onto anti-biotin IgG which was immobilized on microtiter wells. Reaction mixtures containing europium-labeled antiprogesterone antibody complexed sequentially with progesterone in standards or serum samples and with the betatype anti-idiotypic antibody were then reacted with the immobilized alphatype anti-idiotypic antibody. After 30 min of incubation, the fluorescence of europium is measured by time-resolved fluorescence and is proportional to the concentration of progesterone over the range 0-320 nmol/mL. The method demonstrates good sensitivity, precision, and comparability with a direct competitive radioimmunoassay. The idiometric assay for progesterone is suitable for dipstick technology and biosensors.

摘要

基于使用两种识别原抗孕酮抗体高变区内不同表位的抗独特型抗体,开发了一种用于测定血清孕酮的新型非竞争性间接免疫时间分辨荧光免疫测定法。第一种抗独特型抗体,即β型,在结合位点与孕酮竞争原抗孕酮抗体的一个表位。第二种抗独特型抗体,即α型,在孕酮存在的情况下与抗孕酮抗体结合,但由于表位接近,不与β型抗孕酮复合物结合。在当前配置中,生物素化的α型被捕获到固定在微量滴定板孔上的抗生物素IgG上。然后,将含有依次与标准品或血清样品中的孕酮以及β型抗独特型抗体复合的铕标记抗孕酮抗体的反应混合物与固定化的α型抗独特型抗体反应。孵育30分钟后,通过时间分辨荧光测量铕的荧光,其与0至320 nmol/mL范围内的孕酮浓度成正比。该方法具有良好的灵敏度、精密度,且与直接竞争放射免疫测定法具有可比性。孕酮的间接免疫测定法适用于试纸技术和生物传感器。

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