Tsuji M, Shima H, Cunha G R
Department of Anatomy, University of California, San Francisco 94143.
Endocrinology. 1991 Nov;129(5):2289-97. doi: 10.1210/endo-129-5-2289.
Effects of testosterone (T) and insulin on epithelial branching morphogenesis were investigated in cultured seminal vesicles (SVs) of neonatal mice. SVs from 0-day-old male mice were cultured for 0.5-6 days in serum-free chemically defined medium in the presence of T (10(-7) M), insulin (10 micrograms/ml), or T plus insulin or in medium lacking both hormones. Without the addition of both hormones, SVs failed to grow, based on DNA and protein contents, and did not show any epithelial branching morphogenesis. T induced a 2.5-fold increase in protein content in SVs cultured for 6 days and elicited modest epithelial branching morphogenesis. Insulin increased the protein content of cultured SV rudiments as much as T, but failed to elicit epithelial branching morphogenesis. The combination of both hormones induced a 4.3-fold increase in protein content in cultured SVs and elicited more extensive epithelial branching morphogenesis than T alone. Epithelial and mesenchymal DNA contents in SVs declined slightly during the first 12 h of culture in all treatment groups. The epithelial DNA content in SVs grown with insulin alone remained constant thereafter, while that of SVs grown with T alone or in combination with insulin increased 1.2- and 2.6-fold, respectively. In the absence of both hormones, the mesenchymal DNA content remained constant in SVs grown for 6 days after the initial decline in DNA content. In contrast, mesenchymal DNA content was increased to the same degree (1.4-fold) by either T or insulin alone or in combination. The labeling index with [3H]thymidine of SV epithelium and mesenchyme grown under the hormonal conditions described above corroborated the results of epithelial and mesenchymal DNA contents. These data indicate that insulin by itself has no effect on epithelial proliferation and branching morphogenesis in the neonatal mouse SV, but, instead, amplifies the morphogenetic and proliferative effects of androgen on the developing mouse SV, thus eliciting extensive branching morphogenesis. Both insulin and T have a slight (nonsynergistic) effect on proliferation of SV mesenchyme. Analysis of androgen metabolism in developing mouse SVs indicated that dihydrotestosterone was the major product when T was used as substrate in SVs grown under all hormonal conditions. The rate of DHT production per 100 mg protein was not significantly different among the different treatment groups. Higher levels of 5 alpha-androstane-3 alpha,17 beta-diol were detected in SVs grown in the absence vs. the presence of T regardless of the presence or absence of insulin.(ABSTRACT TRUNCATED AT 400 WORDS)
在新生小鼠的精囊(SVs)培养物中研究了睾酮(T)和胰岛素对上皮分支形态发生的影响。将0日龄雄性小鼠的精囊在无血清化学限定培养基中培养0.5 - 6天,培养基中分别添加T(10⁻⁷M)、胰岛素(10微克/毫升)、T加胰岛素或不添加这两种激素。不添加这两种激素时,基于DNA和蛋白质含量,精囊无法生长,且未表现出任何上皮分支形态发生。T使培养6天的精囊中蛋白质含量增加了2.5倍,并引发了适度的上皮分支形态发生。胰岛素使培养的精囊原基蛋白质含量增加程度与T相同,但未能引发上皮分支形态发生。两种激素联合使用使培养的精囊中蛋白质含量增加了4.3倍,且引发了比单独使用T更广泛的上皮分支形态发生。在所有处理组中,培养的最初12小时内,精囊上皮和间充质的DNA含量略有下降。单独用胰岛素培养的精囊中上皮DNA含量此后保持恒定,而单独用T或T与胰岛素联合培养的精囊中上皮DNA含量分别增加了1.2倍和2.6倍。在不添加两种激素的情况下,DNA含量最初下降后,培养6天的精囊中,间充质DNA含量保持恒定。相反,单独使用T或胰岛素或两者联合使用,间充质DNA含量均增加到相同程度(1.4倍)。在上述激素条件下培养的精囊上皮和间充质的[³H]胸腺嘧啶核苷标记指数证实了上皮和间充质DNA含量的结果。这些数据表明,胰岛素本身对新生小鼠精囊上皮的增殖和分支形态发生没有影响,而是放大了雄激素对发育中的小鼠精囊的形态发生和增殖作用,从而引发广泛的分支形态发生。胰岛素和T对精囊间充质的增殖均有轻微(非协同)作用。对发育中的小鼠精囊雄激素代谢的分析表明,在所有激素条件下培养的精囊中,以T为底物时,二氢睾酮是主要产物。不同处理组每100毫克蛋白质中二氢睾酮的产生速率无显著差异。无论有无胰岛素,在无T与有T的情况下培养的精囊中,均检测到较高水平的5α - 雄甾烷 - 3α,17β - 二醇。(摘要截于400字)
