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雄激素刺激后大鼠腹侧前列腺信使核糖核酸含量的特异性变化。来自醛缩酶信使核糖核酸合成的证据。

Specific changes in the messenger ribonucleic acid content of the rat ventral prostate gland after androgenic stimulation. Evidence from the synthesis of aldolase messenger ribonucleic acid.

作者信息

Mainwaring W I, Mangan F R, Irving R A, Jones D A

出版信息

Biochem J. 1974 Nov;144(2):413-26. doi: 10.1042/bj1440413.

Abstract
  1. Aldolase was selected as a suitable marker for following the androgenic regulation of mRNA synthesis in the prostate gland. 2. Antibodies raised in rabbits against crystalline prostate aldolase were used to monitor the synthesis of this androgen-induced enzyme after hormonal stimulation of castrated animals, by using procedures in vivo and in vitro for the translation of prostate poly(A)-rich mRNA. 3. After androgenic stimulation in vivo the poly(A)-rich mRNA was isolated from the prostate gland and other tissues of castrated rats, and added to a protein-synthesizing system in vitro derived from Krebs II ascites-tumour cells. By using this approach it was found that androgens regulate the synthesis of aldolase mRNA in a highly tissue-specific manner. Stimulation of aldolase mRNA synthesis reached a maximum after 8h of androgenic treatment and then declined. 4. The androgenic control of aldolase mRNA synthesis was also investigated in vivo. After treatment of castrated animals with various steroids in vivo [(35)S]methionine was injected directly into the prostate gland, and labelled aldolase was selectively precipitated from isolated polyribosomes with anti-aldolase serum. The regulation of aldolase mRNA synthesis in the prostate gland was stringently steroid-specific and could only be evoked by androgens. After a single injection of testosterone, aldolase synthesis reached a maximum after 16h of hormonal stimulation and then declined. 5. Although androgens exert significant control over transcriptional processes in the prostate gland, and appear to regulate the synthesis of aldolase mRNA de novo, the possibility exists for additional means of control at the translational level of aldolase synthesis. The results are discussed in the context of the overall mechanism of action of androgens.
摘要
  1. 醛缩酶被选为追踪前列腺中mRNA合成雄激素调节的合适标志物。2. 用针对结晶前列腺醛缩酶的兔抗体制剂,通过体内和体外翻译前列腺富含多聚腺苷酸(poly(A))的mRNA的方法,监测去势动物激素刺激后这种雄激素诱导酶的合成。3. 体内雄激素刺激后,从去势大鼠的前列腺和其他组织中分离出富含多聚腺苷酸的mRNA,并添加到源自克雷布斯II腹水瘤细胞的体外蛋白质合成系统中。通过这种方法发现,雄激素以高度组织特异性的方式调节醛缩酶mRNA的合成。雄激素处理8小时后,醛缩酶mRNA合成的刺激达到最大值,然后下降。4. 还在体内研究了醛缩酶mRNA合成的雄激素控制。给去势动物体内注射各种类固醇后,将[35S]甲硫氨酸直接注入前列腺,并用抗醛缩酶血清从分离的多核糖体中选择性沉淀标记的醛缩酶。前列腺中醛缩酶mRNA合成的调节严格具有类固醇特异性,且只能由雄激素诱发。单次注射睾酮后,激素刺激16小时后醛缩酶合成达到最大值,然后下降。5. 尽管雄激素对前列腺中的转录过程有显著控制作用,并且似乎从头调节醛缩酶mRNA的合成,但在醛缩酶合成的翻译水平上存在额外控制手段的可能性。在雄激素作用的整体机制背景下讨论了这些结果。
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/050c/1168510/4a80ce85e18f/biochemj00569-0249-a.jpg

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