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首页> 外文期刊>Biology of Reproduction: Offical Journal of the Society for the Study of Reproduction >Cryopreservation of mouse spermatogonial stem cells in dimethylsulfoxide and polyethylene glycol.
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Cryopreservation of mouse spermatogonial stem cells in dimethylsulfoxide and polyethylene glycol.

机译:二甲基硫氧化物和聚乙二醇中小鼠精子干细胞的冷冻保存。

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摘要

Assisted reproductive techniques involving isolation, culture, and transplantation of spermatogonial stem cells (SSCs) have the potential to create transgenic livestock and to treat male infertility caused by cancer treatments such as chemotherapy or radiation. Because stem cells may need to be preserved for several years before reintroduction to the patients' testes, efficient SSC cryopreservation techniques need to be developed. SSCs can reinitiate spermatogenesis in recipient testes after freezing; however, optimal cryopreservation protocols have not been identified. The objective of this study was to develop an efficient cryopreservation method for SSCs using permeable cryoprotectant agents (PCAs) or additive cryoprotectant agents (ACAs). To identify an efficient cryopreservation method, populations of mouse testis cells enriched for SSCs were cultured in vitro and frozen using conventional freezing media containing various PCAs or ACAs for 1 wk or 1, 3, 6, 12, or 24 mo. Additionally, various molecular weights and concentrations of polyethylene glycol (PEG) were evaluated. Recovery rate, culture potential, and stem cell activity were significantly greater for cells frozen in 2.5% PEG with a molecular weight of 1000 compared to other treatment groups. These cells also retained the ability to colonize recipient testes, generate normal spermatogenesis, and contribute to viable offspring. The systematic analysis of many cryoprotectant agents indicates that 2.5% PEG (molecular weight 1000) is the most effective agent for efficient SSC cryopreservation.
机译:涉及分离,培养和移植精子干细胞(SSCs)的辅助生殖技术具有产生转基因牲畜并治疗由癌症处理(如化疗或辐射)引起的男性不孕症。因为在对患者的睾丸重新调节之前可能需要保持干细胞几年,所以需要开发有效的SSC冷冻保存技术。 SSCs可以在冻结后重新调节受体睾丸的精子发生;但是,尚未确定最佳冷冻保存协议。本研究的目的是使用可渗透的冷冻保护剂(PCA)或添加剂冷冻保护剂(ACAS)来开发一种高效的冷冻保存方法。为了鉴定有效的冷冻保存方法,使用含有各种PCA或ACA的常规冷冻介质培养富含SSCs的小鼠睾丸细胞的群体培养,并将其含有各种PCA或ACAS为1WK或1,3,6,12或24mo。另外,评价各种分子量和聚乙二醇(PEG)的浓度。对于在2.5%PEG中冷冻的细胞,与其他治疗组相比,在2.5%PEG中冷冻的细胞,培养率,培养潜力和干细胞活性显着更大。这些细胞还保留了殖民化接受者测试的能力,产生正常的精子发生,并有助于可行的后代。对许多冷冻保护剂的系统分析表明2.5%PEG(分子量1000)是有效的SSC冷冻保存的最有效剂。

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