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大鼠前列腺蛋白。II. 去势诱导的前列腺腹叶退化过程中新蛋白的合成。

Proteins of the rat prostate. II. Synthesis of new proteins in the ventral lobe during castration-induced regression.

作者信息

Lee C, Sensibar J A

机构信息

Department of Urology, Northwestern University Medical School, Chicago IL 60611.

出版信息

J Urol. 1987 Oct;138(4):903-8. doi: 10.1016/s0022-5347(17)43413-6.

Abstract

Ventral prostates from adult Sprague-Dawley rats at different days postcastration were cut into one to two mm.3 pieces and incubated in medium containing S35-methionine (100 uCi/ml.) at 37C under 95% oxygen and 5% carbon dioxide for four hours. The incubated tissues were subjected to two-dimensional electrophoresis and radiofluorography. Over 100 spots were developed in the fluorograms. Three groups of spots, representing cytoskeletal proteins, androgen-dependent proteins and castration-induced proteins, were further evaluated by a computer-based densitometer. The level of densitometry absorption is proportional to the amount of radioactivity in each spot. The synthesis of cytoskeletal proteins, such as actin and tropomyosin, were relatively constant throughout the course of prostatic regression. The rate of synthesis of androgen-dependent proteins declined rapidly from a high level of synthesis before castration to a non-detectable level by Day 3 postcastration. However, three proteins, which were either not synthesized (spot G and spot H) or synthesized at a very low level (spot I) before castration, were the major proteins synthesized by the prostate during early stages of its regression. The rate of synthesis of these proteins reached a peak by Day 4 postcastration, declined rapidly and remained at a low level thereafter. The respective molecular weights and isoelectric points for these three proteins were 33 Kd and 7.2 for spot G, 38 Kd and 5.3 for spot H and 64 Kd and 6.0 for spot I. Previous findings showed that prostatic regression in rats was associated with a surge of activities in proteolytic enzymes which peaked five to six days postcastration. The peak of synthesis of three proteins noted in the present study, therefore, preceded the peak of activities of proteolytic enzymes in the regressing prostate by one to two days. Testosterone replacement to animals at the time of castration prevented the synthesis of these proteins in the prostate. Since the synthesis of these three proteins in the ventral prostate is induced by androgen-depletion resulted from castration, they are considered as the castration-induced proteins.

摘要

将成年Sprague-Dawley大鼠在去势后不同天数的腹侧前列腺切成1至2立方毫米的小块,并在含有S35-甲硫氨酸(100微居里/毫升)的培养基中,于37℃、95%氧气和5%二氧化碳条件下孵育4小时。将孵育后的组织进行二维电泳和放射自显影。在放射自显影片上出现了100多个斑点。通过基于计算机的密度计对代表细胞骨架蛋白、雄激素依赖性蛋白和去势诱导蛋白的三组斑点进行进一步评估。密度测定吸收水平与每个斑点中的放射性量成正比。在前列腺退化过程中,细胞骨架蛋白如肌动蛋白和原肌球蛋白的合成相对恒定。雄激素依赖性蛋白的合成速率从去势前的高水平迅速下降,到去势后第3天降至不可检测水平。然而,三种在去势前未合成(斑点G和斑点H)或合成水平极低(斑点I)的蛋白质,是前列腺在退化早期合成的主要蛋白质。这些蛋白质的合成速率在去势后第4天达到峰值,随后迅速下降并维持在低水平。这三种蛋白质各自的分子量和等电点分别为:斑点G为33千道尔顿和7.2,斑点H为38千道尔顿和5.3,斑点I为64千道尔顿和6.0。先前的研究结果表明,大鼠前列腺退化与蛋白水解酶活性激增有关,该活性在去势后5至6天达到峰值。因此,本研究中观察到的三种蛋白质合成峰值比退化前列腺中蛋白水解酶活性峰值提前1至2天。在去势时给动物补充睾酮可阻止前列腺中这些蛋白质的合成。由于腹侧前列腺中这三种蛋白质的合成是由去势导致的雄激素耗竭诱导的,它们被视为去势诱导蛋白。

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