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去势对大鼠精囊分泌蛋白IV合成的影响。

Effect of castration on the synthesis of seminal vesicle secretory protein IV in the rat.

作者信息

Ostrowski M C, Kistler M K, Kistler W S

出版信息

Biochemistry. 1982 Jul 20;21(15):3525-9. doi: 10.1021/bi00258a001.

Abstract

The effects of castration on the synthesis (accumulation) of a major seminal vesicle secretory protein (SVS IV) were examined in young adult rats. In vitro incorporation of labeled amino acids into SVS IV by minced tissue was monitored by immunological methods. Castration resulted in a large decrease in the differential synthesis of SVS IV. A significant decrease in the relative incorporation of isotope into SVS IV was evident within 3 days of castration, and by 4 weeks relative incorporation dropped some 30-fold. These changes took place in the presence of a large generalized decline in protein synthesis so that incorporation into SVS IV on an organ basis decreased by over 200-fold. SVS IV messenger RNA levels were estimated by RNA excess solution hybridization using a cloned cDNA probe. Relative message levels declined after castration in harmony with the declines in SVS IV synthesis. SVS IV mRNA was decreased by a relative factor of approximately 20 and an absolute factor of approximately 200 in long-term (40-day) castrates. Accordingly, the seminal vesicle conforms to the general pattern of steroid regulated systems in which hormone withdrawal leads to differential decreases in the steady-state pool size for specific mRNAs. The seminal vesicle is unusual, however, in that a prolonged period is required for maximum differential effects to occur.

摘要

在成年幼鼠中研究了去势对精囊主要分泌蛋白(SVS IV)合成(积累)的影响。通过免疫方法监测切碎组织将标记氨基酸体外掺入SVS IV的情况。去势导致SVS IV差异合成大幅下降。去势后3天内,同位素相对掺入SVS IV显著下降,到4周时相对掺入下降约30倍。这些变化发生在蛋白质合成普遍大幅下降的情况下,因此以器官为基础计算,掺入SVS IV的量减少了200多倍。使用克隆的cDNA探针通过RNA过量溶液杂交估计SVS IV信使RNA水平。去势后相对信使水平下降,与SVS IV合成的下降一致。在长期(40天)去势的大鼠中,SVS IV mRNA相对下降约20倍,绝对下降约200倍。因此,精囊符合类固醇调节系统的一般模式,即激素撤离导致特定mRNA稳态池大小的差异减少。然而,精囊不同寻常之处在于,需要较长时间才能产生最大的差异效应。

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