Effects of canine bone marrow stromal cells after different stages of mineralization on the differentiation, pro⁃ liferation of canine periodontal ligament stem cells

JIN Zhenyu; ZHANG Zhihong

doi:10.12016/j.issn.2096⁃1456.2018.11.003

口腔疾病防治 (Nov 2018)

Effects of canine bone marrow stromal cells after different stages of mineralization on the differentiation, pro⁃ liferation of canine periodontal ligament stem cells

JIN Zhenyu,
ZHANG Zhihong

Affiliations

JIN Zhenyu: Center of Stomatology, The first affiliated hospital of USTC (Anhui Provincial Hospital)
ZHANG Zhihong: Center of Stomatology, The first affiliated hospital of USTC (Anhui Provincial Hospital)

DOI: https://doi.org/10.12016/j.issn.2096⁃1456.2018.11.003
Journal volume & issue: Vol. 26, no. 11
pp. 699 – 705

Abstract

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Objective To investigate the inductive effects of canine periodontal ligament stem cells (PDLSCs) co⁃ cultured with canine disparate differentiating⁃period iliac bone marrow stromal cells (I⁃BMSCs). Methods Purified PDLSCs were isolated by in vitro culture of cBMSCs and flow cytometry. Third⁃generation PDLSCs were obtained, and conditioned culture medium derived fromiliac bone marrow stromal cells (I⁃BMSCs⁃CM) was added as indicated for co⁃ culture of PDLSCs. As the control group, pure uninduced PDLSCs were routinely cultured in DMEM culture medium containing 15%FBS. The experimental groups included the I⁃BMSCs⁃CM, I⁃BMSCs⁃CM⁃10ds and I⁃BMSCs⁃CM⁃15ds groups. The I⁃BMSCs⁃CM group consisted of PDLSCs induced by I⁃BMSCs, the I⁃BMSCs⁃CM⁃10ds group consisted of PDLSCs induced by I⁃BMSCs after osteogenic induction for 10 days, and the I⁃BMSCs⁃CM⁃15ds group consisted of PDLSCs induced by I⁃BMSCs after osteogenic induction for 15 days. The cocultured PDLSCs were examined via the MTT assay. Total mRNA and protein were prepared at 3 and 7 days. The mRNA expression levels of runt⁃related tran⁃ scription factor 2(Runx2), special AT⁃rich sequence binding protein 2(Satb2) and osteocalcin (OCN) were measured by qRT ⁃ PCR. The protein expression levels of Satb2, Runx2 and OCN were detected by Western blot. Results The PDLSCs showed a spindle⁃like morphology. While the BMSC⁃conditioned media increased PDLSCs proliferation, the media conditioned by BMSCs allowed to differentiate for 15 days (I⁃BMSCs⁃CM⁃15days) significantly enhanced PDLSCs proliferation (F＝342.8, P＝0.017). The expression levels of the analyzed genes were upregulated in the coculture groups, and the protein expression levels of Satb2, Runx2 and OCN were higher in the test groups than in the control group at 7 days. At the protein level, I⁃BMSCs⁃CM⁃15days upregulated the expression of Satb2 by 3.04⁃fold (FSatb2＝ 24.48, P＝0.014), Runx2 by 5.1⁃fold (FRunx2＝12.25, P < 0.001), and OCN by 3.67⁃fold (FOCN＝18.35, P＝0.022). Con⁃ clusion The conditioned medium of I⁃BMSCs may enhance the proliferation of PDLSCs, and that of terminally differen⁃ tiated bone cells probably triggered the osteogenesis of PDLSCs, suggesting important implications for periodontal engi⁃ neering.

Published in 口腔疾病防治

ISSN: 2096-1456 (Print)
Publisher: Editorial Department of Journal of Prevention and Treatment for Stomatological Diseases
Country of publisher: China
LCC subjects: Medicine
Website: http://www.kqjbfz.com/EN/2096-1456/home.shtml

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