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斑马鱼精原干细胞在培养中分化为功能性精子。

Differentiation of zebrafish spermatogonial stem cells to functional sperm in culture.

作者信息

Kawasaki Toshihiro, Siegfried Kellee R, Sakai Noriyoshi

机构信息

Genetic Strains Research Center, National Institute of Genetics, Mishima 411-8540, Japan.

University of Massachusetts Boston, Biology Department, Boston, MA 02125, USA.

出版信息

Development. 2016 Feb 15;143(4):566-74. doi: 10.1242/dev.129643. Epub 2015 Dec 30.

DOI:10.1242/dev.129643
PMID:26718005
Abstract

Molecular dissection and chemical screening on a complex process such as spermatogenesis could be facilitated by cell culture approaches that allow easy access for experimental manipulation and live imaging of specific molecules; however, technical limitations have thus far prevented the complete reconstruction of spermatogenic events in cell culture. Here, we describe the production of functional sperm from self-renewing spermatogonial stem cells (SSCs) in cell culture conditions, using zebrafish testicular hyperplasia cells that accumulate early stage spermatogonia. By serially transplanting hyperplasias into immunodeficient rag1 mutant zebrafish, we succeeded in long-term maintenance and efficient production of starting material for SSC culture. Through improvements of culture conditions, we achieved efficient propagation of SSCs derived from the hyperplasia. When SSCs that underwent the SSC-propagating step for 1 month were transferred onto Sertoli feeder cells, they differentiated into functional sperm that gave rise to offspring. Oxygen at the concentration of air proved to be detrimental for sperm differentiation from SSCs, but not for propagation of SSCs. These results indicate that the whole spermatogenic process can be represented in cell culture in zebrafish, facilitating analyses of the molecular mechanisms of spermatogenesis in vertebrates.

摘要

细胞培养方法有助于对精子发生等复杂过程进行分子剖析和化学筛选,因为这些方法便于进行实验操作并对特定分子进行实时成像;然而,技术限制迄今阻碍了在细胞培养中完全重建精子发生事件。在此,我们描述了在细胞培养条件下,利用积累早期精原细胞的斑马鱼睾丸增生细胞,从自我更新的精原干细胞(SSCs)产生功能性精子的过程。通过将增生组织连续移植到免疫缺陷的rag1突变斑马鱼中,我们成功地长期维持并高效生产了用于SSC培养的起始材料。通过改善培养条件,我们实现了源自增生组织的SSCs的高效增殖。当经过1个月SSC增殖步骤的SSCs转移到支持细胞饲养层上时,它们分化为功能性精子并产生了后代。事实证明,空气浓度的氧气对SSCs分化为精子有害,但对SSCs的增殖无害。这些结果表明,斑马鱼的整个精子发生过程可以在细胞培养中呈现,这有助于分析脊椎动物精子发生的分子机制。

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