VEGFR2-dependent Angiogenic Capacity of Pericyte-like Dental Pulp Stem Cells

牙髓干细胞 周细胞 血管生成 细胞生物学 基质凝胶 化学 干细胞 间质细胞 CD146号 内皮干细胞 生物 癌症研究 体外 生物化学 川地34
作者
Kajohnkiart Janebodin,Yachang Zeng,Worakanya Buranaphatthana,Nicholas Ieronimakis,Morayma Reyes
出处
期刊:Journal of Dental Research [SAGE Publishing]
卷期号:92 (6): 524-531 被引量:96
标识
DOI:10.1177/0022034513485599
摘要

Dental pulp stem cells (DPSCs) have previously demonstrated potential pericyte-like topography and function. However, the mechanisms regulating their pericyte function are still unknown. In this study, murine DPSC angiogenic and pericyte function were investigated. Tie2-GFP mouse DPSCs were negative for GFP, indicating the absence of endothelial cells in DPSC cultures. Endothelial cells co-cultured with DPSCs formed more mature in vitro tube-like structures as compared with those co-cultured with bone marrow stromal cells (BMSCs). Many DPSCs were located adjacent to vascular tubes, assuming a pericyte location. Subcutaneous DPSC transplants in mice with matrigel (MG) (DPSC-MG) induced more vessel formation than BMSC-MG. Soluble Flt (sFlt), an angiogenic inhibitor that binds VEGF-A, significantly decreased the amount of blood vessels in DPSC-MG, but not in BMSC-MG. sFlt inhibited VEGFR2 and downstream ERK signaling in DPSCs. Similar to sFlt inhibition, VEGFR2 knockdown in DPSCs resulted in down-regulation of Vegfa, Vegf receptors, and EphrinB2 and decreased angiogenic induction of DPSCs in vivo. Therefore, the capacity of DPSCs to induce angiogenesis is VEGFR2-dependent. DPSCs enhance angiogenesis by secreting VEGF ligands and associating with vessels resembling pericyte-like cells. This study provides first insights into the mechanism(s) of DPSC angiogenic induction and their function as pericytes, crucial aspects for DPSC use in tissue regeneration.
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