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Co-option of the bZIP transcription factor Vrille as the activator of Doublesex1 in environmental sex determination of the crustacean Daphnia magna

机译:bZIP转录因子Vrille作为Doublesex1的激活剂在甲壳类水蚤(Daphnia magna)的环境性别测定中的选择

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摘要

Divergence of upstream regulatory pathways of the transcription factor Doublesex (Dsx) serves as a basis for evolution of sex-determining mechanisms in animals. However, little is known about the regulation of Dsx in environmental sex determination. In the crustacean Daphnia magna, environmental sex determination is implemented by male-specific expression of the Dsx ortholog, Dsx1. Transcriptional regulation of Dsx1 comprises at least three phases during embryogenesis: non-sex-specific initiation, male-specific up-regulation, and its maintenance. Herein, we demonstrate that the male-specific up-regulation is controlled by the bZIP transcription factor, Vrille (Vri), an ortholog of the circadian clock genes—Drosophila Vri and mammalian E4BP4/NFIL3. Sequence analysis of the Dsx1 promoter/enhancer revealed a conserved element among two Daphnia species (D. magna and D. pulex), which contains a potential enhancer harboring a consensus Vri binding site overlapped with a consensus Dsx binding site. Besides non-sex-specific expression of Vri in late embryos, we found male-specific expression in early gastrula before the Dsx1 up-regulation phase begins. Knockdown of Vri in male embryos showed reduction of Dsx1 expression. In addition, transient overexpression of Vri in early female embryos up-regulated the expression of Dsx1 and induced male-specific trait. Targeted mutagenesis using CRISPR/Cas9 disrupted the enhancer on genome in males, which led to the reduction of Dsx1 expression. These results indicate that Vri was co-opted as a transcriptional activator of Dsx1 in environmental sex determination of D. magna. The data suggests the remarkably plastic nature of gene regulatory network in sex determination.
机译:转录因子Doublesex(Dsx)上游调节途径的差异是动物性别决定机制进化的基础。但是,关于环境性别确定中Dsx的调控知之甚少。在甲壳类水蚤(Daphnia magna)中,环境性别的确定是通过Dsx直系同源基因Dsx1的雄性特异性表达来实现的。 Dsx1的转录调控在胚胎发生过程中至少包括三个阶段:非性别特异性启动,男性特异性上调及其维持。本文中,我们证明了雄性特异性上调受bZIP转录因子Vrille(Vri),昼夜节律基因Drosophila Vri和哺乳动物E4BP4 / NFIL3的直系同源基因控制。 Dsx1启动子/增强子的序列分析揭示了两个水蚤物种(D. magna和D. pulex )中的保守元件,其中包含潜在的增强子,该潜在增强子带有共有的Vri结合位点,与共有的Dsx结合重叠现场。除了 Vri 在晚期胚胎中的非性别特异性表达外,我们还发现在 Dsx1 上调阶段开始之前,胃早期的雄性特异性表达。敲除雄性胚胎中的 Vri 显示出 Dsx1 表达的减少。此外,早期雌性胚胎中瞬时表达的 Vri 上调了 Dsx1 的表达并诱导了雄性特质。使用CRISPR / Cas9进行定向诱变破坏了男性基因组上的增强子,从而导致 Dsx1 表达的减少。这些结果表明,在 D 的环境性别测定中, Vri 被选作 Dsx1 的转录激活因子。 magna 。数据表明性别调控中基因调控网络的显着可塑性。

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