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睾酮对大鼠精囊中信使核糖核酸和蛋白质合成的影响。

Effects of testosterone on messenger ribonucleic acid and protein synthesis in rat seminal vesicle.

作者信息

Higgins S J, Burchell J M

出版信息

Biochem J. 1978 Aug 15;174(2):543-51. doi: 10.1042/bj1740543.

Abstract

In a previous report [Higgins et al. (1976) Biochem. J.158, 271-282] we described the effects of alterations in androgen status on the synthesis of two basic secretory proteins of the rat seminal vesicle. In the present paper we examine the effects of testosterone on the activity of mRNA in the seminal vesicle. Total cellular poly(A)-rich RNA was isolated and translated in a cell-free system prepared from wheat germ. Translation products were separated on denaturing polyacrylamide gels and the protein bands corresponding to the two basic secretory proteins were identified immunologically. Incorporation of radioactive methionine into these bands was taken as a measure of the individual mRNA activities. Total mRNA activity was estimated by radioactivity in total acid-precipitable material. The results show that 1 to 2 weeks after castration the activities of mRNA molecules for the basic secretory proteins were decreased 10-20-fold on a tissue basis. Testosterone given in vivo rapidly and substantially restores mRNA activity to normal. Since these changes correlate closely with variations in the rates of synthesis of the secretory proteins in whole cells it suggests that androgenic steroids control protein synthesis chiefly via mRNA availability. In this respect their action resembles those of other steroid hormones acting in other systems. However, these effects of testosterone on the mRNA molecules for the major secretory proteins could not be distinguished from those on total mRNA. Thus the proportion of the total mRNA population accounted for by the two specific mRNA molecules showed less than a 2-fold variation with androgen status. Similarly the two secretory proteins always accounted for 25-33% of general protein synthesis. This is in sharp contrast with the markedly differential effects of other steroid hormones controlling synthesis of major proteins in other well-studied systems. We interpret our results as indicating that testosterone regulates the mRNA population of the seminal vesicle as a whole.

摘要

在之前的一篇报告中[希金斯等人(1976年),《生物化学杂志》158卷,271 - 282页],我们描述了雄激素状态改变对大鼠精囊两种碱性分泌蛋白合成的影响。在本文中,我们研究了睾酮对精囊mRNA活性的影响。分离出细胞总富含多聚腺苷酸(poly(A))的RNA,并在由小麦胚芽制备的无细胞系统中进行翻译。翻译产物在变性聚丙烯酰胺凝胶上分离,通过免疫鉴定与两种碱性分泌蛋白相对应的蛋白条带。将放射性甲硫氨酸掺入这些条带中作为各个mRNA活性的指标。通过总酸沉淀物质中的放射性来估计总mRNA活性。结果表明,去势后1至2周,碱性分泌蛋白的mRNA分子活性在组织水平上降低了10至20倍。体内给予睾酮能迅速且显著地将mRNA活性恢复至正常。由于这些变化与全细胞中分泌蛋白合成速率的变化密切相关,这表明雄激素类固醇主要通过mRNA的可利用性来控制蛋白质合成。在这方面,它们的作用类似于在其他系统中起作用的其他类固醇激素。然而,睾酮对主要分泌蛋白的mRNA分子的这些影响与对总mRNA的影响无法区分。因此,这两种特定mRNA分子在总mRNA群体中所占比例随雄激素状态的变化小于2倍。同样,这两种分泌蛋白在一般蛋白质合成中始终占25% - 33%。这与其他类固醇激素在其他深入研究的系统中对主要蛋白质合成的显著差异作用形成鲜明对比。我们将结果解释为表明睾酮整体上调节精囊的mRNA群体。

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