Huang Stephanie, Sartini Becky L, Parks John E
Department of Animal Science, 201 Morrison Hall, Cornell University, Ithaca, NY 14853, United States.
Anim Reprod Sci. 2008 Jan 15;103(1-2):1-12. doi: 10.1016/j.anireprosci.2006.11.018. Epub 2006 Dec 1.
Xenografting of testis explants into recipient mice has resulted in successful restoration of spermatogenesis in several species. Most studies have utilized neonatal donor tissue, although a few have used prepubertal testes. In Holstein bulls, prepubertal development of the testis occurs between 16 and 32 weeks of age. The purpose of the present study was to determine the optimal age during prepubertal development of Holstein bulls for testis grafting. Explants of testis tissue from Holstein bulls between 12 and 32 weeks of age (2 bulls/age; 6 ages) were subcutaneously grafted into castrated or intact immunocompromised mice (n=8/age), then recovered after 75 and 173 days (n=4 mice/grafting period) and evaluated histologically for spermatogenic progression. Seminiferous tubules were assigned a score based on the most advanced type of germ cell present within the tubule and the average for all tubules scored (n=25) within an explant was calculated. Scores for all explants per mouse (n=6) were averaged to give a single spermatogenic progression score per mouse. No difference in spermatogenic progression of grafts between intact and castrated recipients was observed. Spermatocytes were observed in testis grafts from bulls of all ages 75 days post-grafting. At 173 days, the spermatogenic progression score for explants derived from 20 weeks bulls was greater than all ages except 12 weeks donors (p<0.05), with 8% of tubules containing spermatids. Donor material from bulls older than 20 weeks had lesser spermatogenic progression scores largely attributed to the greater number of atrophic tubules in grafts from older donors. Grafts from 28 and 32 weeks donors showed signs of degeneration by 75 days post-grafting, with 30 and 55% atrophic tubules, respectively, and lesser spermatogenic efficiency scores. By 173 days post-grafting, 72% of tubules in explants from 32 weeks donors were atrophic. The results of the present study suggest that the early stages of prepubertal development are optimal for testis grafting while advanced spermatogenesis in the donor tissue prior to grafting had a negative effect on graft development. Spermatogenesis within the grafts apparently needs to be re-established by spermatogonial stem cells or early spermatogonia.
将睾丸外植体移植到受体小鼠体内已成功恢复了几个物种的精子发生。大多数研究使用新生供体组织,不过也有一些研究使用青春期前的睾丸。在荷斯坦公牛中,睾丸的青春期前发育发生在16至32周龄之间。本研究的目的是确定荷斯坦公牛青春期前发育过程中进行睾丸移植的最佳年龄。将12至32周龄荷斯坦公牛的睾丸组织外植体(每个年龄2头公牛;共6个年龄)皮下移植到去势或完整的免疫受损小鼠体内(每个年龄n = 8只),然后在75天和173天后取出(每个移植期n = 4只小鼠),并进行组织学评估以确定精子发生进展情况。根据曲细精管内存在的最成熟生殖细胞类型为曲细精管打分,并计算每个外植体中所有打分曲细精管(n = 25)的平均值。计算每只小鼠(n = 6)所有外植体的得分平均值,得出每只小鼠的单个精子发生进展得分。未观察到完整受体和去势受体之间移植体精子发生进展的差异。移植后75天,所有年龄公牛的睾丸移植体中均观察到精母细胞。在173天时,来自20周龄公牛的外植体的精子发生进展得分高于除12周龄供体以外的所有年龄(p<0.05),有8%的曲细精管含有精子细胞。来自20周龄以上公牛的供体材料的精子发生进展得分较低,这主要归因于来自年龄较大供体的移植体中萎缩曲细精管数量较多。来自28周龄和32周龄供体的移植体在移植后75天时出现退化迹象,萎缩曲细精管分别为30%和55%,精子发生效率得分较低。到移植后173天时,来自32周龄供体的外植体中72%的曲细精管萎缩。本研究结果表明,青春期前发育的早期阶段是睾丸移植的最佳时期,而移植前供体组织中晚期精子发生对移植体发育有负面影响。移植体内的精子发生显然需要由精原干细胞或早期精原细胞重新建立。
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