Ultrasound Stimulation of Different Dental Stem Cell Populations: Role of Mitogen-activated Protein Kinase Signaling

被引：51

作者：

Gao, Qianhua ^{[1
]}

Walmsley, A. Damien ^{[1
]}

Cooper, Paul R. ^{[1
]}

Scheven, Ben A. ^{[1
]}

机构：

[1] Univ Birmingham, Sch Dent, Coll Med & Dent Sci, Birmingham B4 6NN, W Midlands, England

来源：

JOURNAL OF ENDODONTICS | 2016年 / 42卷 / 03期

关键词：

Bone marrow mesenchymal stem cells; cell proliferation; dental pulp stem cells; dental tissue regeneration; low-intensity pulsed ultrasound; mitogen-activated protein kinase signaling; mesenchymal stem cells; periodontal ligament-derived stem cells; ultrasound; INTENSITY PULSED ULTRASOUND; LOW-FREQUENCY ULTRASOUND; ODONTOBLAST-LIKE CELLS; IN-VIVO; CHONDROGENIC DIFFERENTIATION; PERIODONTAL-LIGAMENT; BONE; PROLIFERATION; CULTURE; VITRO;

D O I：

10.1016/j.joen.2015.12.019

中图分类号：

R78 [口腔科学];

学科分类号：

1003 ;

摘要：

Introduction: Mesenchymal stem cells (MSCs) from dental tissues may respond to low-intensity pulsed ultrasound (LIPUS) treatment, potentially providing a therapeutic approach to promoting dental tissue regeneration. This work aimed to compare LIPUS effects on the proliferation and MAPK signaling in MSCs from rodent dental pulp stem cells (DPSCs) compared with MSCs from periodontal ligament stem cells (PDLSCs) and bone marrow stem cells (BMSCs). Methods: Isolated MSCs were treated with 1-MHz LIPUS at an intensity of 250 or 750 mW/cm(2) for 5 or 20 minutes. Cell proliferation was evaluated by 5-bromo-2-deoxyuridine (BrdU) staining after 24 hours of culture following a single LIPUS treatment. Specific ELISAs were used to determine the total and activated p38, ERK1/2, and JNK MAPK signaling proteins up to 4 hours after treatment. Selective MAPK inhibitors PD98059 (ERK1/2), SB203580 (p38), and SP600125 (JNK) were used to determine the role of activation of the particular MAPK pathways. Results: The proliferation of all MSC types was significantly increased after LIPUS treatment. LIPUS at a 750-mW/cm(2) dose induced the greatest effects on DPSCs. BMSC proliferation was stimulated in equal measures by both intensities, whereas 250 mW/cm(2) LIPUS exposure exerted maximum effects on PDLSCs. ERK1/2 was activated immediately in DPSCs after treatment. Concomitantly, DPSC proliferation was specifically modulated by ERK1/2 inhibition, whereas p38 and JNK inhibition exerted no effects. In BMSCs, JNK MAPK signaling was LIPUS activated, and the increase in proliferation was blocked by specific inhibition of the JNK pathway. In PDLSCs, JNK MAPK signaling was activated immediately after LIPUS, whereas p-p38 MAPK increased significantly in these cells 4 hours after exposure. Correspondingly, JNK and p38 inhibition modulated LIPUS-stimulated PDLSC proliferation. Conclusions: LIPUS promoted MSC proliferation in an intensity and cell-specific dependent manner via activation of distinct MAPK pathways.

引用

页码：425 / 431

页数：7