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小鼠精囊中雄激素调节蛋白的发育模式。

Developmental pattern of androgen-regulated proteins in seminal vesicles from the mouse.

作者信息

Normand T, Jean-Faucher C, Jean C

机构信息

Physiologie Comparée et Endocrinologie, CNRS UA 360, Université Blaise Pascal, Aubiére, France.

出版信息

Int J Androl. 1989 Jun;12(3):219-30. doi: 10.1111/j.1365-2605.1989.tb01307.x.

Abstract

Proteins from secretions or homogenates of mice seminal vesicles were analysed by polyacrylamide gel electrophoresis. In homogenates about 15 bands were differentially induced with molecular weights (MW's) of 12, 13, 14, 15, 15.5, 71, 120 and 140 kD, or repressed molecular weights of 12.5, 14.3, 28, 30, 53, 73, 90-105 kD). The effects of castration were reversed by testosterone and dihydrotestosterone but not by oestradiol, progesterone or corticosterone. When the androgen-dependence of proteins was investigated using radioactive methionine the protein spectra showed that about 12 bands with molecular weights of 13, 13.7, 14, 15, 15.5, 16, 20.5, 24, 37, 38.5, 56, 68, 96 and 180 kD were differentially induced or repressed by androgens. Of the induced proteins, those with low molecular weight (12-15.5 kD) were accumulated in significant amounts between 20 days and 30 days, coincident with the pubertal increase of androgens in the seminal vesicles. Those induced proteins with high molecular weight (71, 120 and 140 kD) appeared between 40 days and 60 days. The androgen-repressed proteins were strongly evident in immature males, but disappeared after day 40.

摘要

通过聚丙烯酰胺凝胶电泳分析了小鼠精囊分泌物或匀浆中的蛋白质。在匀浆中,约15条带的诱导或抑制存在差异,其分子量(MW)分别为12、13、14、15、15.5、71、120和140kD,或被抑制的分子量为12.5、14.3、28、30、53、73、90 - 105kD。去势的影响可被睾酮和双氢睾酮逆转,但不能被雌二醇、孕酮或皮质酮逆转。当使用放射性甲硫氨酸研究蛋白质的雄激素依赖性时,蛋白质谱显示,约12条分子量为13、13.7、14、15、15.5、16、20.5、24、37、38.5、56、68、96和180kD的带被雄激素差异诱导或抑制。在诱导的蛋白质中,低分子量(12 - 15.5kD)的蛋白质在20天至30天之间大量积累,这与精囊中雄激素的青春期增加相一致。那些高分子量(71、120和140kD)的诱导蛋白质在40天至60天之间出现。雄激素抑制的蛋白质在未成熟雄性中明显可见,但在40天后消失。

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