Androgen-induced changes in Leydig cell ultrastructure and steroidogenesis in juvenile African catfish, Clarias gariepinus

被引:0
|
作者
J. E. B. Cavaco
B. van Blijswijk
J. F. Leatherland
H. J. Th. Goos
R. W. Schulz
机构
[1] Research Group for Comparative Endocrinology,
[2] Faculty of Biology,undefined
[3] Utrecht University,undefined
[4] Padualaan 8,undefined
[5] 3584 CH Utrecht,undefined
[6] The Netherlands e-mail: r.w.schulz@bio.uu.nl; Tel: +31 30 2533046; Fax: +31 30 2532837,undefined
[7] Department of Biomedical Sciences,undefined
[8] Ontario Veterinary College,undefined
[9] University of Guelph,undefined
[10] Guelph,undefined
[11] ON N1G 2W1,undefined
[12] Canada,undefined
[13] Universidade do Algarve,undefined
[14] UCTRA,undefined
[15] Centro de Ciências do Mar,undefined
[16] Campus de Gambelas,undefined
[17] P-8000 Faro,undefined
[18] Portugal,undefined
来源
Cell and Tissue Research | 1999年 / 297卷
关键词
Key words Teleost fish; Puberty; Testes; Sex steroids; Ultrastructure; Steroidogenesis; Clarias gariepinus (Teleostei);
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学科分类号
摘要
The present report focuses on the mechanism(s) involved in the steroid-induced decrease of androgen production in immature African catfish testes that was observed in previous studies. Juvenile animals were implanted with Silastic pellets containing different 11-oxygenated androgens (11-ketotestosterone, KT; 11β- hydroxyandrostenedione, OHA; 11-ketoandrostenedione, KA), testosterone (T) or estradiol-17β (E2). Control groups received steroid-free pellets. Two weeks later, testis tissue fragments were either incubated with increasing concentrations of catfish luteinizing hormone (LH), or incubated with [3H]-pregnenolone ([3H]-P5) or [3H]-androstenedione ([3H]-A). Tissue fragments were also prepared for the quantitative assessment of Leydig cell morphology. Most of the parameters studied were not affected significantly by implantation of E2. Implantation of all androgens inhibited both the basal and the LH-stimulated androgen secretory capacity in vitro. This was associated with a reduced size of the Leydig cells and loss of half of their mitochondria. The studies on the metabolism of tritiated steroid hormones indicated that steroidogenic steps prior to 11β-hydroxylation, probably C17–20 lyase activity, were affected by all androgens. Although the effects of 11-oxygenated androgens and T on Leydig cells were mostly similar, previous work showed that only the 11-oxygenated androgens stimulated spermatogenesis, suggesting that distinct mechanisms of action are used by 11-oxygenated androgens and T. These mechanisms, however, seem to merge on the same target(s) to impair Leydig cell androgen production. Such a negative feedback mechanism may be of relevance in the context of the decline in androgen secretion per milligram testis tissue that accompanies the first wave of spermatogenesis in pubertal African catfish.
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页码:291 / 299
页数:8
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