Weinbauer G F, Schubert J, Yeung C H, Rosiepen G, Nieschlag E
Institute of Reproductive Medicine, the University, Münster, Germany.
J Endocrinol. 1998 Jan;156(1):23-34. doi: 10.1677/joe.0.1560023.
Meiosis constitutes a crucial phase of spermatogenesis since the recombination of genetic information and production of haploid round spermatids need to be achieved. Although it is well established that gonadotrophic hormones are required for completion of the spermatogenic process, little is known about the dynamic and kinetic aspects of development of spermatocytes into spermatids and its endocrine control in the primate. In this study, S-phase germ cells were labelled using 5-bromodeoxyuridine (BrdU) incorporation and were then followed throughout meiosis under normal conditions and following GnRH antagonist (ANT)-induced gonadotrophin withdrawal in a nonhuman primate model, the cynomolgus monkey (Macaca fascicularis). Adult animals received either vehicle (VEH, n = 4) or the ANT cetrorelix (n = 5) throughout 25 days. On day 7 all animals received a bolus injection of BrdU. A biopsy was performed after 3 h, one testis was removed 9 days later (day 16 of treatment) and the other testis after 18 days (day 25 of treatment). Serum testosterone and inhibin levels, and testis weight were reduced (P < 0.05) by ANT treatment. BrdU localized to pachytene spermatocytes 9 days after BrdU and to round spermatids 18 days after BrdU in both groups, demonstrating that BrdU-labelled pachytene spermatocytes had undergone meiosis. Flow cytometric analysis revealed that the relative number and number per testis of BrdU-tagged 2C and 4C cells were reduced significantly (P < 0.05) within 16 days of ANT treatment. Numbers of 1C cells were lowered by day 25. The cell ratio for 1C:4C was similar with VEH and ANT (P > 0.05). These findings indicate that ANT reduced the number of cells available for meiosis but did not alter the rate of transition into round spermatids. Unexpectedly, however, the stage-dependent progression of BrdU-tagged round spermatids was significantly (P < 0.05) retarded under ANT as seen from the frequency of tubules containing BrdU-labelled round spermatids. The average duration of spermatogenic cycle was slightly prolonged (9.8 days in the VEH group and 10.8 days in the ANT group (P = 0.09)). Since no atypical germ cell associations could be found, it remains unclear whether this slight prolongation is entirely due to altered spermatid progression or whether earlier phases are affected. We conclude for the nonhuman primate that (1) BrdU-labelling of premeiotic germ cells is suitable for tracing their meiotic transition into postmeiotic cells, (2) unlike in the rat, gonadotrophin suppression initially affects premeiotic cell proliferation and thus the number of cells available for meiosis, (3) the meiotic process continues quantitatively despite gonadotrophin deficiency and (4) prolonged gonadotrophin deficiency might alter the timing of germ cell development.
减数分裂是精子发生的关键阶段,因为需要完成遗传信息的重组和单倍体圆形精子细胞的产生。尽管促性腺激素是精子发生过程完成所必需的这一点已得到充分证实,但在灵长类动物中,关于精母细胞发育成精子细胞的动态和动力学方面及其内分泌控制却知之甚少。在本研究中,使用5-溴脱氧尿苷(BrdU)掺入法标记S期生殖细胞,然后在正常条件下以及在非人灵长类动物模型食蟹猴(猕猴属)中,在GnRH拮抗剂(ANT)诱导促性腺激素撤退后,对整个减数分裂过程进行跟踪观察。成年动物在25天内接受溶剂对照(VEH,n = 4)或ANT西曲瑞克(n = 5)处理。在第7天,所有动物接受一次BrdU推注。3小时后进行活检,9天后(治疗第16天)切除一侧睾丸,18天后(治疗第25天)切除另一侧睾丸。ANT处理使血清睾酮和抑制素水平以及睾丸重量降低(P < 0.05)。在两组中,BrdU在BrdU处理9天后定位于粗线期精母细胞,18天后定位于圆形精子细胞,表明BrdU标记的粗线期精母细胞已经经历了减数分裂。流式细胞术分析显示,在ANT处理的16天内,BrdU标记的2C和4C细胞的相对数量和每睾丸数量显著减少(P < 0.05)。到第25天,1C细胞数量下降。1C:4C的细胞比例在VEH组和ANT组中相似(P > 0.05)。这些发现表明,ANT减少了可用于减数分裂的细胞数量,但没有改变向圆形精子细胞转变的速率。然而,出乎意料的是,从含有BrdU标记的圆形精子细胞的小管频率来看,ANT处理下BrdU标记的圆形精子细胞的阶段依赖性进展显著延迟(P < 0.05)。生精周期的平均持续时间略有延长(VEH组为9.8天,ANT组为10.8天(P = 0.09))。由于未发现非典型生殖细胞关联,目前尚不清楚这种轻微延长是否完全是由于精子细胞进展改变,还是早期阶段也受到影响。对于非人灵长类动物,我们得出以下结论:(1)减数分裂前生殖细胞的BrdU标记适用于追踪它们向减数分裂后细胞的减数分裂转变;(2)与大鼠不同,促性腺激素抑制最初影响减数分裂前细胞增殖,从而影响可用于减数分裂的细胞数量;(3)尽管促性腺激素缺乏,减数分裂过程在数量上仍继续进行;(4)长期促性腺激素缺乏可能会改变生殖细胞发育的时间。
