Zhu Ximei, Zhao YiMeng, Bai Xiaofan, Dong Qiannan, Tian Chunli, Sun Ruilin, Yan Congjuan, Ruan Jianping, Liu Zhongbo, Gao Jianghong
Key Laboratory of Shaanxi Province for Craniofacial Precision Medicine Research, College of Stomatology, Xi'an Jiaotong University, Xi'an, Shaanxi, 710004, China.
Center of Oral Public Health, College of Stomatology, Xi'an Jiaotong University, Xi'an, Shaanxi, 710004, China.
Stem Cell Res Ther. 2025 Apr 12;16(1):173. doi: 10.1186/s13287-025-04294-6.
Ameloblasts present a promising avenue for the investigation of enamel and tooth regeneration. Previous protocols for directing the differentiation of human embryonic stem cells (hESCs) into dental epithelial (DE) cells involving the need for additional cells, conditional medium, and the use of costly cytokines. Importantly, ameloblasts have not been generated from hESCs in previous studies. Hence, we aimed to identify defined differentiation conditions that would solely utilize small molecules to achieve the production of ameloblasts.
We developed a three-step strategy entailing the progression of hESCs through non-neural ectoderm (NNE) and DE to generate functional ameloblasts in vitro. Initially, the NNE fate was induced from hESCs using a 6-day differentiation protocol with 1 µmol/L Retinoic acid (RA). Subsequently, the NNE lineage was differentiated into DE by employing a combination of 1 µmol/L LDN193189 (a BMP signaling inhibitor) and 1 µmol/L XAV939 (a WNT signaling inhibitor). In the final phase, 3 µmol/L CHIR99021 (a WNT signaling activator) and 2 µmol/L DAPT (a NOTCH signaling inhibitor) were utilized to achieve the fate of ameloblasts from DE cells. Three-dimensional cultures were investigated to enhance the ameloblast differentiation ability of the induced DE cells. Quantitative reverse transcription polymerase chain reaction (qRT-PCR) and immunofluorescence were conducted to assess the expression of lineage-specific markers. Alizarin Red S (ARS) staining was performed to evaluate the formation of mineralization nodules.
The application of RA facilitated the efficient generation of NNE within a six-day period. Subsequently, upon stimulation with LDN193189 and XAV939, a notable emergence of DE cells was observed on the eighth days. By the tenth day, ameloblast-like cells derived from hESCs were generated. Upon cultivation in spheroids, these cells exhibited elevated levels of ameloblast markers AMBN and AMELX expression, suggesting that spheroid culture augments the differentiation of ameloblasts.
We established an efficient small molecule-based method to differentiate hESCs into ameloblast-like cells through the concerted modulation of RA, BMP, WNT, and NOTCH signaling pathways, potentially advancing research in enamel and tooth regeneration.
成釉细胞为牙釉质和牙齿再生研究提供了一条很有前景的途径。以往将人类胚胎干细胞(hESC)诱导分化为牙上皮(DE)细胞的方案需要额外的细胞、条件培养基以及使用昂贵的细胞因子。重要的是,以往研究中尚未从hESC生成成釉细胞。因此,我们旨在确定仅利用小分子来实现成釉细胞生成的明确分化条件。
我们制定了一个三步策略,使hESC依次经过非神经外胚层(NNE)和DE阶段,以在体外生成功能性成釉细胞。最初,使用含1 μmol/L视黄酸(RA)的6天分化方案从hESC诱导NNE命运。随后,通过联合使用1 μmol/L LDN193189(一种骨形态发生蛋白信号抑制剂)和1 μmol/L XAV939(一种WNT信号抑制剂)将NNE谱系分化为DE。在最后阶段,使用3 μmol/L CHIR99021(一种WNT信号激活剂)和2 μmol/L DAPT(一种NOTCH信号抑制剂)使DE细胞实现成釉细胞命运。研究了三维培养以增强诱导的DE细胞的成釉细胞分化能力。进行定量逆转录聚合酶链反应(qRT-PCR)和免疫荧光以评估谱系特异性标志物的表达。进行茜素红S(ARS)染色以评估矿化结节的形成。
RA的应用促进了6天内NNE的高效生成。随后,在用LDN193189和XAV939刺激后,在第8天观察到DE细胞显著出现。到第10天,生成了源自hESC的成釉样细胞。在球体中培养时,这些细胞显示出成釉细胞标志物AMBN和AMELX表达水平升高,表明球体培养增强了成釉细胞的分化。
我们建立了一种基于小分子的有效方法,通过协同调节RA、骨形态发生蛋白、WNT和NOTCH信号通路将hESC分化为成釉样细胞,这可能推动牙釉质和牙齿再生的研究。
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