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生殖系干细胞分化需要秀丽隐杆线虫中细胞命运调节因子GLD-1的区域控制。

Germline Stem Cell Differentiation Entails Regional Control of Cell Fate Regulator GLD-1 in Caenorhabditis elegans.

作者信息

Brenner John L, Schedl Tim

机构信息

Department of Genetics, Washington University School of Medicine, St. Louis, Missouri 63110.

Department of Genetics, Washington University School of Medicine, St. Louis, Missouri 63110

出版信息

Genetics. 2016 Mar;202(3):1085-103. doi: 10.1534/genetics.115.185678. Epub 2016 Jan 12.

Abstract

Germline stem cell differentiation in Caenorhabditis elegans is controlled by glp-1 Notch signaling. Cell fate regulator GLD-1 is sufficient to induce meiotic entry and expressed at a high level during meiotic prophase, inhibiting mitotic gene activity. glp-1 signaling and other regulators control GLD-1 levels post-transcriptionally (low in stem cells, high in meiotic prophase), but many aspects of GLD-1 regulation are uncharacterized, including the link between glp-1-mediated transcriptional control and post-transcriptional GLD-1 regulation. We established a sensitive assay to quantify GLD-1 levels across an ∼35-cell diameter field, where distal germline stem cells differentiate proximally into meiotic prophase cells in the adult C. elegans hermaphrodite, and applied the approach to mutants in known or proposed GLD-1 regulators. In wild-type GLD-1 levels elevated ∼20-fold in a sigmoidal pattern. We found that two direct transcriptional targets of glp-1 signaling, lst-1 and sygl-1, were individually required for repression of GLD-1. We determined that lst-1 and sygl-1 act in the same genetic pathway as known GLD-1 translational repressor fbf-1, while lst-1 also acts in parallel to fbf-1, linking glp-1-mediated transcriptional control and post-transcriptional GLD-1 repression. Additionally, we estimated the position in wild-type gonads where germ cells irreversibly commit to meiotic development based on GLD-1 levels in worms where glp-1 activity was manipulated to cause an irreversible fate switch. Analysis of known repressors and activators, as well as modeling the sigmoidal accumulation pattern, indicated that regulation of GLD-1 levels is largely regional, which we integrated with the current view of germline stem cell differentiation.

摘要

秀丽隐杆线虫中的生殖系干细胞分化由glp-1 Notch信号通路控制。细胞命运调节因子GLD-1足以诱导减数分裂进入,并在减数分裂前期高水平表达,抑制有丝分裂基因活性。glp-1信号通路和其他调节因子在转录后控制GLD-1水平(干细胞中低,减数分裂前期高),但GLD-1调节的许多方面尚未明确,包括glp-1介导的转录控制与转录后GLD-1调节之间的联系。我们建立了一种灵敏的检测方法,以量化约35个细胞直径范围内的GLD-1水平,在成年秀丽隐杆线虫雌雄同体中,远端生殖系干细胞向近端分化为减数分裂前期细胞,并将该方法应用于已知或推测的GLD-1调节因子的突变体。在野生型中,GLD-1水平以S形模式升高约20倍。我们发现glp-1信号通路的两个直接转录靶标lst-1和sygl-1分别是抑制GLD-1所必需的。我们确定lst-1和sygl-1与已知的GLD-1翻译抑制因子fbf-1在同一遗传途径中起作用,而lst-1也与fbf-1平行起作用,将glp-1介导的转录控制与转录后GLD-1抑制联系起来。此外,我们根据操纵glp-1活性以导致不可逆命运转换的线虫中GLD-1水平,估计了野生型性腺中生殖细胞不可逆地进入减数分裂发育的位置。对已知抑制因子和激活因子的分析,以及对S形积累模式的建模表明,GLD-1水平调节在很大程度上是区域性的,我们将其与当前的生殖系干细胞分化观点相结合。

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本文引用的文献

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