Generation and characterization of a Dkk4-Cre knock-in mouse line

H. Khatif, H. Bazzi
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Abstract

Ectodermal appendages in mammals, such as teeth, mammary glands, sweat glands and hair follicles, are generated during embryogenesis through a series of mesenchymal-epithelial interactions. Canonical Wnt signaling and its inhibitors are implicated in the early steps of ectodermal appendage development and patterning. To study the activation dynamics of the Wnt target and inhibitor Dickkopf4 (Dkk4) in ectodermal appendages, we used CRSIPR/Cas9 to generate a Dkk4-Cre knock-in mouse (Mus musculus) line, where the Cre recombinase cDNA replaces the expression of endogenous Dkk4. Using Cre reporters, the Dkk4-Cre activity was evident at the prospective sites of ectodermal appendages, overlapping with the Dkk4 mRNA expression. Unexpectedly, a predominantly mesenchymal cell population in the embryo posterior also showed Dkk4-Cre activity. Lineage-tracing suggested that these cells are likely derived from a few Dkk4-Cre-expressing cells in the epiblast at early gastrulation. Finally, our analyses of Dkk4-Cre-expressing cells in developing hair follicle epithelial placodes revealed intra- and inter-placodal cellular heterogeneity, supporting emerging data on the positional and transcriptional variability in placodes. Collectively, we propose the new Dkk4-Cre knock-in mouse line as a suitable model to study Wnt and DKK4 inhibitor dynamics in early mouse development and ectodermal appendage morphogenesis.
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Dkk4-Cre敲入小鼠细胞系的产生和表征
哺乳动物的外胚层附属物,如牙齿、乳腺、汗腺和毛囊,是在胚胎发生过程中通过一系列间充质-上皮相互作用产生的。典型Wnt信号及其抑制剂与外胚层附属物发育和模式的早期步骤有关。为了研究Wnt靶点和抑制剂Dickkopf4 (Dkk4)在外胚层附属物中的激活动力学,我们使用CRSIPR/Cas9技术生成了Dkk4-Cre敲入小鼠(Mus musus)系,其中Cre重组酶cDNA取代了内源性Dkk4的表达。使用Cre报告器,Dkk4-Cre活性在外胚层附属物的预期位点明显,与Dkk4 mRNA表达重叠。出乎意料的是,胚胎后部主要的间充质细胞群也显示出Dkk4-Cre活性。谱系追踪表明,这些细胞可能来源于早期原肠胚形成时外胚层中少数表达dkk4 - cre的细胞。最后,我们对发育中的毛囊上皮基板中表达dkk4 - cre的细胞的分析揭示了基板内和基板间的细胞异质性,支持了关于基板位置和转录变异性的新数据。总之,我们提出新的DKK4 - cre敲入小鼠系作为合适的模型来研究Wnt和DKK4抑制剂在小鼠早期发育和外胚层附属物形态发生中的动态。
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