Small Molecules Promote the Rapid Generation of Dental Epithelial Cells from Human-Induced Pluripotent Stem Cells

被引:2
作者
Zhu, Ximei [1 ,2 ]
Li, Yue [1 ,2 ]
Dong, Qiannan [1 ,2 ]
Tian, Chunli [2 ]
Gong, Jing [3 ]
Bai, Xiaofan [3 ]
Ruan, Jianping [1 ,2 ]
Gao, Jianghong [1 ,2 ]
机构
[1] Xi An Jiao Tong Univ, Coll Stomatol, Key Lab Shaanxi Prov Craniofacial Precis Med Res, Xian 710004, Peoples R China
[2] Xi An Jiao Tong Univ, Coll Stomatol, Ctr Oral Publ Hlth, Xian 710004, Peoples R China
[3] Xi An Jiao Tong Univ, Coll Stomatol, Dept Pediat Dent, Xian 710004, Peoples R China
关键词
human-induced pluripotent stem cells; dental epithelial; small molecules; spheroid; RETINOIC ACID; DIFFERENTIATION; EXPRESSION; ENAMEL; FATE;
D O I
10.3390/ijms25084138
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
Human-induced pluripotent stem cells (hiPSCs) offer a promising source for generating dental epithelial (DE) cells. Whereas the existing differentiation protocols were time-consuming and relied heavily on growth factors, herein, we developed a three-step protocol to convert hiPSCs into DE cells in 8 days. In the first phase, hiPSCs were differentiated into non-neural ectoderm using SU5402 (an FGF signaling inhibitor). The second phase involved differentiating non-neural ectoderm into pan-placodal ectoderm and simultaneously inducing the formation of oral ectoderm (OE) using LDN193189 (a BMP signaling inhibitor) and purmorphamine (a SHH signaling activator). In the final phase, OE cells were differentiated into DE through the application of Purmorphamine, XAV939 (a WNT signaling inhibitor), and BMP4. qRT-PCR and immunostaining were performed to examine the expression of lineage-specific markers. ARS staining was performed to evaluate the formation of the mineralization nodule. The expression of PITX2, SP6, and AMBN, the emergence of mineralization nodules, and the enhanced expression of AMBN and AMELX in spheroid culture implied the generation of DE cells. This study delineates the developmental signaling pathways and uses small molecules to streamline the induction of hiPSCs into DE cells. Our findings present a simplified and quicker method for generating DE cells, contributing valuable insights for dental regeneration and dental disease research.
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页数:14
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