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青春期前人类精原干细胞和小鼠生殖细胞具有保守的生殖干细胞调控分子的基因表达。

Prepubertal human spermatogonia and mouse gonocytes share conserved gene expression of germline stem cell regulatory molecules.

机构信息

Department of Animal Biology, School of Veterinary Medicine, University of Pennsylvania, Philadelphia, PA 19104, USA.

出版信息

Proc Natl Acad Sci U S A. 2009 Dec 22;106(51):21672-7. doi: 10.1073/pnas.0912432106. Epub 2009 Dec 14.

Abstract

In the human testis, beginning at approximately 2 months of age, gonocytes are replaced by adult dark (Ad) and pale (Ap) spermatogonia that make up the spermatogonial stem cell (SSC) pool. In mice, the SSC pool arises from gonocytes approximately 6 days after birth. During puberty in both species, complete spermatogenesis is established by cells that differentiate from SSCs. Essentially pure populations of prepubertal human spermatogonia and mouse gonocytes were selected from testis biopsies and validated by confirming the presence of specific marker proteins in cells. Stem cell potential of germ cells was demonstrated by transplantation to mouse testes, following which the cells migrated to the basement membrane of the seminiferous tubule and were maintained similar to SSCs. Differential gene expression profiles generated between germ cells and testis somatic cells demonstrated that expression of genes previously identified as SSC and spermatogonial-specific markers (e.g., zinc-finger and BTB-domain containing 16, ZBTB16) was greatly elevated in both human spermatogonia and mouse gonocytes compared to somatic cells. Several genes were expressed at significantly higher levels in germ cells of both species. Most importantly, genes known to be essential for mouse SSC self-renewal (e.g., Ret proto-oncogene, Ret; GDNF-family receptor alpha1, Gfr alpha1; and B-cell CLL/lymphoma 6, member B, Bcl6b) were more highly expressed in both prepubertal human spermatogonia and mouse gonocytes than in somatic cells. The results indicate remarkable conservation of gene expression, notably for self-renewal genes, in these prepubertal germline cells between two species that diverged phylogenetically approximately 75 million years ago.

摘要

在人类睾丸中,大约从 2 个月龄开始,生殖细胞被成年暗(Ad)和淡(Ap)精原细胞取代,这些细胞构成了精原干细胞(SSC)池。在小鼠中,SSC 池大约在出生后 6 天由生殖细胞产生。在这两个物种的青春期,完全的精子发生是由从 SSCs 分化而来的细胞建立的。从睾丸活检中选择了基本纯的未成熟人类精原细胞和小鼠生殖细胞,并通过确认细胞中存在特定标记蛋白来验证其正确性。通过将这些细胞移植到小鼠睾丸中,证明了生殖细胞的干细胞潜力,随后这些细胞迁移到生精小管的基膜,并保持类似于 SSCs 的状态。生殖细胞与睾丸体细胞之间的差异基因表达谱表明,以前被鉴定为 SSC 和精原细胞特异性标记物(例如,锌指和 BTB 结构域包含蛋白 16,ZBTB16)的基因在人类精原细胞和小鼠生殖细胞中的表达水平大大高于体细胞。两种物种的生殖细胞中有几个基因的表达水平显著升高。最重要的是,在这两个物种的生殖细胞中,已知对小鼠 SSC 自我更新至关重要的基因(例如,Ret 原癌基因,Ret;GDNF 家族受体 alpha1,Gfr alpha1;和 B 细胞 CLL/淋巴瘤 6,成员 B,Bcl6b)的表达水平高于体细胞。这些结果表明,在这两个物种的未成熟生殖细胞中,基因表达存在显著的保守性,特别是在自我更新基因方面,这两个物种在大约 7500 万年前在系统发育上已经分化。

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