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产前和产后光周期对黑线毛足鼠(Phodopus sungorus sungorus)精子发生发育的影响。

Effect of prenatal and postnatal photoperiod on spermatogenic development in the Djungarian hamster (Phodopus sungorus sungorus).

作者信息

van Haaster L H, van Eerdenburg F J, de Rooij D G

机构信息

Department of Cell Biology, Medical School, Utrecht University, The Netherlands.

出版信息

J Reprod Fertil. 1993 Jan;97(1):223-32. doi: 10.1530/jrf.0.0970223.

Abstract

The effect of the pre- and postnatal daylength on the start of spermatogenesis and further testicular development from day 4 up to day 127 was investigated in Djungarian hamsters. Hamsters were either gestated under long (16 h light:8 h dark) photoperiod and reared under long or short (4 h light:20 h dark) photoperiod after birth (L/L and L/S hamsters, respectively), or gestated under short photoperiod and transferred to long photoperiod after birth (S/L hamsters). In L/L and L/S hamsters, spermatogenesis started between day 4 and day 5 (day of birth = day 1), when the first gonocytes entered the S-phase. A, Intermediate and B spermatogonia were first observed on days 6, 8 and 9, respectively. The proliferation pattern of gonocytes and Sertoli cells, studied between day 4 and day 9, did not differ between L/L and L/S hamsters. Hence, the duration of the postnatal photoperiod had no effect on the start of spermatogenesis. The first effect of postnatal photoperiod on spermatogenic development was observed on day 15, when testis weights and tubular diameters were reduced in L/S animals. From day 22 onwards, spermatogenesis was arrested mainly at the mid-pachytene stage, no tubular lumen was formed, and the number of preleptotene spermatocytes was reduced. The ultimate number of Sertoli cells per testis was not affected by postnatal short photoperiod. The duration of the prenatal photoperiod had a clear effect on spermatogenesis after birth. In S/L hamsters, the number of gonocytes per tubular cross-section was reduced on day 4 and 4.5. Gonocyte proliferation was reduced on day 5 and spermatogenesis started one day later. Consequently, A and Intermediate spermatogonia appeared on day 7 and 9, respectively. Sertoli cell proliferation was also shifted to later ages, but the ultimate number of Sertoli cells did not differ from L/L or L/S hamsters. From day 29 onwards, the number of preleptotene spermatocytes was increased in S/L hamsters, indicating that the Sertoli cells in these animals could support more germinal cells. In conclusion, a short postnatal photoperiod does not affect spermatogenesis before day 15 after birth, when further testicular development becomes arrested. A short prenatal photoperiod delays the start of spermatogenesis by one day, alters the proliferation pattern of Sertoli cells, and from day 29 onwards, enables the Sertoli cells to support more germinal cells. The duration of the pre- and postnatal photoperiod did not affect the ultimate number of Sertoli cells.

摘要

在侏儒仓鼠中,研究了产前和产后光周期对精子发生起始以及从出生后第4天到第127天睾丸进一步发育的影响。仓鼠要么在长光周期(16小时光照:8小时黑暗)下妊娠,出生后在长光周期或短光周期(4小时光照:20小时黑暗)下饲养(分别为L/L和L/S仓鼠),要么在短光周期下妊娠,出生后转移到长光周期(S/L仓鼠)。在L/L和L/S仓鼠中,精子发生在出生后第4天到第5天(出生日=第1天)开始,此时第一批生殖母细胞进入S期。A、中间型和B型精原细胞分别在第6天、第8天和第9天首次观察到。在第4天到第9天研究的生殖母细胞和支持细胞的增殖模式在L/L和L/S仓鼠之间没有差异。因此,产后光周期的持续时间对精子发生的起始没有影响。产后光周期对精子发生发育的第一个影响在第15天观察到,此时L/S动物的睾丸重量和管径减小。从第22天起,精子发生主要停滞在粗线期中期,没有形成管腔,前细线期精母细胞数量减少。每个睾丸中支持细胞的最终数量不受产后短光周期的影响。产前光周期的持续时间对出生后的精子发生有明显影响。在S/L仓鼠中,每个管状横截面上的生殖母细胞数量在第4天和4.5天减少。生殖母细胞增殖在第5天减少,精子发生开始时间推迟一天。因此,A型和中间型精原细胞分别在第7天和第9天出现。支持细胞增殖也推迟到较晚年龄,但支持细胞的最终数量与L/L或L/S仓鼠没有差异。从第29天起,S/L仓鼠中前细线期精母细胞数量增加,表明这些动物中的支持细胞能够支持更多的生殖细胞。总之,产后短光周期在出生后第15天之前不影响精子发生,之后睾丸进一步发育停滞。产前短光周期使精子发生起始推迟一天,改变支持细胞的增殖模式,并且从第29天起,使支持细胞能够支持更多的生殖细胞。产前和产后光周期的持续时间不影响支持细胞的最终数量。

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