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视黄酸对小鼠雄性生殖细胞进入减数分裂的直接影响。

Direct effects of retinoic acid on entry of fetal male germ cells into meiosis in mice.

机构信息

Institute for Biogenesis Research, John A. Burns School of Medicine, University of Hawaii, Honolulu, Hawaii 96813, USA.

出版信息

Biol Reprod. 2010 Dec;83(6):1056-63. doi: 10.1095/biolreprod.110.085787. Epub 2010 Sep 8.

Abstract

In both male and female germ cells of mice, retinoic acid (RA) is a meiosis-inducing factor. In the present study, we used a germ cell culture system to examine the direct effects of RA on meiotic initiation in male germ cells at the stage when they normally enter mitotic arrest to determine the extent to which fetal male germ cells can respond to exogenous RA to alter their sex-specific pathway. Male germ cells between 13.5 and 15.5 days postcoitum (dpc) were isolated from Pou5fl-green fluorescent protein transgenic fetuses and cultured with or without RA for up to 6 days. In the absence of RA, male germ cells did not undergo DNA replication and did not enter meiosis in culture. However, in the presence of RA, male germ cells isolated at 13.5 dpc expressed Stra8 and initiated the meiotic process. The ratio of cells entering meiosis gradually decreased as cells were isolated progressively at later stages. By 15.5 dpc, isolated male germ cells lost their ability to respond to RA signaling. These cells remained dispersed as single cells and progressed along the male differentiation pathway, as evidenced by the establishment of male-specific methylation imprints regardless of the presence or absence of RA. We conclude that male germ cells maintain sexual bipotency until 14.5 dpc that can be reversed by the addition of RA. Once male germ cells enter mitotic arrest, however, they appear to be committed irreversibly to the male-specific differentiation pathway even in the presence of exogenously added RA.

摘要

在雄性和雌性小鼠生殖细胞中,视黄酸(RA)是一种减数分裂诱导因子。在本研究中,我们使用生殖细胞培养系统来检测 RA 对处于有丝分裂阻滞阶段的雄性生殖细胞减数分裂起始的直接影响,以确定胎儿雄性生殖细胞在多大程度上可以对外源 RA 作出反应,改变其性别特异性途径。从 Pou5fl-绿色荧光蛋白转基因胎鼠中分离出 13.5 至 15.5 天龄的雄性生殖细胞,并在有或没有 RA 的情况下培养长达 6 天。在没有 RA 的情况下,雄性生殖细胞不会进行 DNA 复制,也不会在培养中进入减数分裂。然而,在 RA 的存在下,在 13.5 天龄时分离的雄性生殖细胞表达 Stra8 并启动减数分裂过程。随着细胞在后期阶段逐渐分离,进入减数分裂的细胞比例逐渐下降。到 15.5 天龄时,分离的雄性生殖细胞失去了对 RA 信号的反应能力。这些细胞仍然作为单个细胞分散存在,并沿着雄性分化途径前进,这一点可以从无论是否存在 RA,雄性特异性甲基化印记的建立得到证明。我们得出结论,雄性生殖细胞在 14.5 天龄之前保持两性潜能,可以通过添加 RA 来逆转。然而,一旦雄性生殖细胞进入有丝分裂阻滞,它们似乎就不可逆地朝着雄性特异性分化途径前进,即使存在外源添加的 RA。

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