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未成年公羊羔的培养和富集睾丸生殖细胞在同种异体受者接受白消安治疗后的体内移植成功。

Successful in vivo Transplantation of Cultured and Enriched Testicular Germ Cells of Pre-Pubertal Bucks to Busulfan-Treated Homologous Recipients.

机构信息

Animal Physiology and Reproduction Division, ICAR-Central Institute for Research on Goats, Mathura, India.

ICAR-National Bureau of Fish Genetic Resources, Lucknow, India.

出版信息

Cells Tissues Organs. 2023;212(3):232-244. doi: 10.1159/000523891. Epub 2022 Mar 4.

DOI:10.1159/000523891
PMID:35249016
Abstract

The objective of the present study was to establish a workable approach for the production of germ cell (GC)-depleted recipient goat model using intra-testicular busulfan treatment and transplantation of cultured and enriched caprine-male GC (cmGCs) into the homologous recipients under ultrasonography (USG) guidance. The evaluation of post-transplantation colonization of donor cmGCs and restoration of the normal architecture of seminiferous tubules (ST) was performed. For this, the cmGCs of pre-pubertal male goats were isolated and enriched by differential platting for culture until the third passage. Thereafter, cells were harvested and further enriched by magnetic-activated cell sorting using rabbit-anti-CD90 antibody. After confirmation of metabolic viability (MTT-assay) and cluster-forming ability (crystal violet staining) of CD90+ cmGCs, the cells were labeled with a lipophilic red-fluorescent dye (PKH26) before transplanted into the recipient male goats by injection directly into the mediastinum testes under USG guidance. The colonization and repopulation of transplanted CD90+ cmGCs into the recipient ST was observed up to 8 weeks post-transplantation. The PKH26-labeled donor cell-derived colonies were identified in enzymatically digested ST and cryosections of recipient testes. Moreover, histochemical analyses revealed the restoration of the normal architecture of ST of recipient testis after GC transplantation. Therefore, the results suggest that the reproductive competence of infertile animals can be restored through mGC therapy and thus the methodology presented herein could be useful to obtain donor mGCs-derived functional male gametes in the recipient animal testis.

摘要

本研究旨在建立一种可行的方法,即在超声引导下,用睾丸内白消安处理和移植培养及富集的山羊雄性生殖细胞(GC),来制备 GC 耗竭的受体山羊模型。评估移植后供体 cmGC 的定植和曲细精管(ST)正常结构的恢复情况。为此,对未成年雄性山羊的 cmGC 进行分离和富集,通过差 plating 进行培养,直到第 3 代。然后,收获细胞并用兔抗 CD90 抗体进行磁激活细胞分选进一步富集。在确认 CD90+cmGC 的代谢活力(MTT 测定)和集落形成能力(结晶紫染色)后,将细胞用亲脂性红色荧光染料(PKH26)标记,然后在超声引导下直接注射到纵隔睾丸中移植到受体雄性山羊体内。观察到移植的 CD90+cmGC 定植和再殖到受体 ST 长达 8 周。在酶消化的 ST 和受体睾丸的冷冻切片中鉴定出 PKH26 标记的供体细胞衍生的集落。此外,组织化学分析显示 GC 移植后受体睾丸 ST 的正常结构得到了恢复。因此,这些结果表明,通过 mGC 治疗可以恢复不育动物的生殖能力,因此本文提出的方法可能有助于在受体动物睾丸中获得供体 mGC 衍生的功能性雄性配子。

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