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人催乳素的液相双位点免疫放射分析

A liquid-phase two-site immunoradiometric assay for human prolactin.

作者信息

Hodgkinson S C, Landon J, Lowry P J

出版信息

Biochem J. 1984 Jan 1;217(1):273-9. doi: 10.1042/bj2170273.

Abstract

The development of a 'two-site' immunoradiometric assay for human prolactin (hPrl) is described. The assay is based on the addition of radio-iodinated sheep anti-hPrl immunoglobulin G (IgG) and rabbit anti-hPrl serum to standards and unknowns followed by 3 h incubation. The use of solid phase reagents was avoided in order to minimize non-specific effects and the time required for reactants to reach equilibrium. Instead, the separation of hPrl-bound and free labelled antibody is achieved by the addition of sheep anti-(rabbit IgG) serum which precipitates bound labelled antibody by complex formation with rabbit anti-hPrl antibodies which are also hPrl-bound. Varying the order of addition of specific antibodies had a pronounced effect on the 'operating range' and sensitivity of resultant assays. This was attributed to competition between labelled and unlabelled antibodies for binding sites on the hPrl molecule. The immunoradiometric assay employing 'simultaneous addition' of specific antibodies was compared to a 'simultaneous addition' hPrl radioimmunoassay developed using the same sheep antiserum as that used to prepare the radioiodinated sheep anti-hPrl IgG. This immunoradiometric assay is characterized by rapid equilibration of reactants, a wide 'operating range' (the precision of dose estimates was less than 10% over the range 8-10000 mU/l), and high sensitivity (2.6 mU/l, 13 pg). In contrast, the hPrl radioimmunoassay required an incubation of 18 h, demonstrated a much reduced 'operating range' (the precision of dose estimates was less than 10% only over the range 25-1500 mU/l) and reduced sensitivity (9.8 mU/l, 49 pg).

摘要

本文描述了一种用于人催乳素(hPrl)的“双位点”免疫放射分析方法的开发。该分析方法是在标准品和未知样品中加入放射性碘化羊抗人催乳素免疫球蛋白G(IgG)和兔抗人催乳素血清,然后孵育3小时。为了尽量减少非特异性效应以及反应物达到平衡所需的时间,避免使用固相试剂。相反,通过加入羊抗(兔IgG)血清来分离与hPrl结合的和游离的标记抗体,该血清通过与也与hPrl结合的兔抗人催乳素抗体形成复合物而沉淀结合的标记抗体。改变特异性抗体的加入顺序对所得分析方法的“检测范围”和灵敏度有显著影响。这归因于标记抗体和未标记抗体在hPrl分子上结合位点的竞争。将采用特异性抗体“同时加入”的免疫放射分析方法与使用与制备放射性碘化羊抗人催乳素IgG相同的羊抗血清开发的“同时加入”hPrl放射免疫分析方法进行了比较。这种免疫放射分析方法的特点是反应物快速平衡、“检测范围”宽(在8 - 10000 mU/l范围内剂量估计的精密度小于10%)和灵敏度高(2.6 mU/l,13 pg)。相比之下,hPrl放射免疫分析需要孵育18小时,其“检测范围”大大减小(仅在25 - 1500 mU/l范围内剂量估计的精密度小于10%)且灵敏度降低(9.8 mU/l,49 pg)。

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