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人血清高分子量催乳素的生化性质:一种催乳素结合蛋白的鉴定

Biochemical nature of high-molecular-weight prolactin of human serum: identification of a prolactin-binding protein.

作者信息

Bulatov A A, Martynov A V, Smirnova N B

机构信息

Endocrinology Research Center, Russian Academy of Medical Sciences, Moscow, Russia.

出版信息

Biochemistry (Mosc). 1997 Sep;62(9):1039-46.

PMID:9457766
Abstract

The biochemical nature of a high-molecular-weight immunoreactive prolactin (HMW-irPRL) prepared by gel filtration of women's sera with predominance of this hormone form was studied. Immunochemical characteristics of HMW-irPRL are different from those of 23 kD prolactin (23 kD-PRL). A protein which specifically and reversibly binds to human [125I]PRL is isolated from the pooled fractions of HMW-irPRL by affinity chromatography on prolactin-Sepharose. According to gel filtration, the binding protein (BP) has molecular weight about 150 kD, and it reversibly binds to protein A immobilized on Sepharose. Analysis of BP by SDS-PAGE resulted in two major protein bands, of 65-70 and approximately 150 kD. Both the bands, when transferred to nitrocellulose, interacted with [125I]protein A. Binding of highly purified human pituitary prolactin to the BP significantly decreased the immunoreactivity of the hormone. The molecular weight of BP and its interaction with protein A and recognition by poly- and monoclonal antibodies against human (but not guinea pig) IgG indicate that BP may be an immunoglobulin. Thus, our data demonstrate that HMW-irPRL is formed by the binding of 23 kD-PRL to a specific serum protein which is probably an anti-prolactin IgG.

摘要

对以这种激素形式为主的女性血清进行凝胶过滤制备的高分子量免疫反应性催乳素(HMW-irPRL)的生化性质进行了研究。HMW-irPRL的免疫化学特性与23kD催乳素(23kD-PRL)不同。通过在催乳素-琼脂糖上进行亲和色谱,从HMW-irPRL的合并级分中分离出一种能特异性且可逆地结合人[125I]PRL的蛋白质。根据凝胶过滤,结合蛋白(BP)的分子量约为150kD,并且它能可逆地结合固定在琼脂糖上的蛋白A。通过SDS-PAGE对BP进行分析,得到两条主要的蛋白带,分别为65 - 70kD和约150kD。当这两条带转移到硝酸纤维素膜上时,它们都与[125I]蛋白A相互作用。高度纯化的人垂体催乳素与BP的结合显著降低了该激素的免疫反应性。BP的分子量及其与蛋白A的相互作用以及针对人(而非豚鼠)IgG的多克隆和单克隆抗体对其的识别表明,BP可能是一种免疫球蛋白。因此,我们的数据表明,HMW-irPRL是由23kD-PRL与一种可能是抗催乳素IgG的特异性血清蛋白结合形成的。

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