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绵羊黄体中催乳激素的受体。I:放射性标记的绵羊催乳素和人生长激素特异性结合的一个主要差异。

Receptors for lactogenic hormones in the ovine corpus luteum. I: A major discrepancy in the specific binding of radiolabelled ovine prolactin and human growth hormone.

作者信息

Bramley T A, Menzies G S, McNeilly A S, Friesen H G

出版信息

J Endocrinol. 1987 Jun;113(3):365-74. doi: 10.1677/joe.0.1130365.

Abstract

The characteristics of the binding of 125I-labelled human GH (hGH) and ovine prolactin (oPRL) were studied in the ovine corpus luteum. Although oPRL is the homologous ligand for sheep lactogenic receptors, its binding was significantly and consistently lower than that of 125I-labelled hGH. This was not due to iodination damage of oPRL since: (1) 125I-labelled oPRL tracers which bound poorly relative to 125I-labelled hGH in the ovine corpus luteum were equipotent in the pig and rat corpus luteum, (2) the differences between 125I-labelled hGH and oPRL binding persisted with tracers of equivalent biopotency and (3) the iodination procedure affected neither oPRL bioactivity in the Nb2 tumour assay nor its binding activity with ovine corpus luteum receptors. Ovine luteal receptors were specific for lactogenic hormones. The specific binding of 125I-labelled hGH or oPRL could be inhibited completely by incubation with either unlabelled hormone, with similar potencies. However, oGH inhibited binding only at much higher concentrations, consistent with its known contamination with oPRL. Moreover, 125I-labelled oGH was not bound specifically to sheep luteal tissue. Fractionation of sheep luteal homogenates on sucrose density gradients (with or without cell-surface membrane perturbation by digitonin) demonstrated that binding of 125I-labelled hGH and 125I-labelled oPRL peaked in the same regions of the gradients, coincident with a number of luteal cell-surface membrane markers. We conclude that the marked discrepancy between the binding of hGH and oPRL tracers by sheep luteal tissue was not due to iodination damage of oPRL, binding of 125I-labelled hGH to somatogenic receptors or differential binding to luteal cell-surface versus intracellular receptors.

摘要

在绵羊黄体中研究了¹²⁵I标记的人生长激素(hGH)和羊催乳素(oPRL)的结合特性。尽管oPRL是绵羊催乳素受体的同源配体,但其结合量显著且持续低于¹²⁵I标记的hGH。这并非由于oPRL的碘化损伤,原因如下:(1)在绵羊黄体中相对于¹²⁵I标记的hGH结合较差的¹²⁵I标记的oPRL示踪剂在猪和大鼠黄体中具有同等效力;(2)¹²⁵I标记的hGH和oPRL结合之间的差异在具有同等生物活性的示踪剂中仍然存在;(3)碘化过程既不影响oPRL在Nb2肿瘤检测中的生物活性,也不影响其与绵羊黄体受体的结合活性。绵羊黄体受体对催乳素激素具有特异性。¹²⁵I标记的hGH或oPRL的特异性结合可以通过与未标记的激素孵育而完全被抑制,且效力相似。然而,oGH仅在高得多的浓度下才抑制结合,这与其已知的被oPRL污染一致。此外,¹²⁵I标记的oGH未特异性结合绵羊黄体组织。在蔗糖密度梯度上对绵羊黄体匀浆进行分级分离(无论有无洋地黄皂苷对细胞表面膜的扰动)表明,¹²⁵I标记的hGH和¹²⁵I标记的oPRL的结合在梯度的相同区域达到峰值,与一些黄体细胞表面膜标记物一致。我们得出结论,绵羊黄体组织对hGH和oPRL示踪剂结合存在显著差异并非由于oPRL的碘化损伤、¹²⁵I标记的hGH与生长激素受体的结合或与黄体细胞表面受体与细胞内受体的差异结合。

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