PER2 regulates odontoblastic differentiation of dental papilla cells in vitro via intracellular ATP content and reactive oxygen species levels

牙乳头 细胞生物学 牙本质形成 成牙本质细胞 化学 活性氧 细胞分化 牙本质涎磷蛋白 下调和上调 碱性磷酸酶 牙本质 生物化学 生物 病理 医学 基因
作者
Haozhen Ma,Xinyue Sheng,Wanting Chen,Hongwen He,Jiawei Liu,Yifan He,Fang Huang
出处
期刊:PeerJ [PeerJ]
卷期号:11: e16489-e16489
标识
DOI:10.7717/peerj.16489
摘要

Background Dental papilla cells (DPCs) are one of the key stem cells for tooth development, eventually forming dentin and pulp. Previous studies have reported that PER2 is expressed in a 24-hour oscillatory pattern in DPCs in vitro . In vivo , PER2 is highly expressed in odontoblasts (which are differentiated from DPCs). However, whether PER2 modulates the odontogenic differentiation of DPCs is uncertain. This research was to identify the function of PER2 in the odontogenic differentiation of DPCs and preliminarily explore its mechanisms. Methods We monitored the expression of PER2 in DPCs differentiated in vivo . We used PER2 overexpression and knockdown studies to assess the role of PER2 in DPC differentiation and performed intracellular ATP content and reactive oxygen species (ROS) assays to further investigate the mechanism. Results PER2 expression was considerably elevated throughout the odontoblastic differentiation of DPCs in vivo . Overexpressing Per2 boosted levels of odontogenic differentiation markers, such as dentin sialophosphoprotein ( Dspp ), dentin matrix protein 1 ( Dmp1 ), and alkaline phosphatase ( Alp ), and enhanced mineralized nodule formation in DPCs. Conversely, the downregulation of Per2 inhibited the differentiation of DPCs. Additionally, downregulating Per2 further affected intracellular ATP content and ROS levels during DPC differentiation. Conclusion Overall, we demonstrated that PER2 positively regulates the odontogenic differentiation of DPCs, and the mechanism may be related to mitochondrial function as shown by intracellular ATP content and ROS levels.
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