異なる細胞培養液における骨芽細胞の骨形成評価ー国際標準法の開発を目指してー

DOI
  • 泉谷 惇
    信州大学 大学院 総合医理工学研究科 生命医工学専攻
  • 上田 勝也
    信州大学 大学院 総合医理工学研究科 生命医工学専攻
  • 馬 闖
    信州大学 大学院 総合医理工学研究科 生命医工学専攻
  • 上芝 洸貴
    信州大学 大学院 総合理工学研究科 生命医工学専攻
  • 羽二生 久夫
    信州大学 先鋭領域融合研究群 バイオメディカル研究所
  • 齋藤 直人
    信州大学 先鋭領域融合研究群 バイオメディカル研究所

書誌事項

タイトル別名
  • Osteogenesis evaluation of osteoblasts in different cell culture media: Towards the development of international standardized methods

抄録

<p>Background: In the early developmental stages of new biomaterials and therapeutic agents targeting the bone, there are cases in which in vitro reproducibility cannot be obtained or there is discrepancy with the results of in vivo experiments. Therefore, we examined the effects of different in vitro culture medium conditions, which could be a cause of such variability, on the evaluation of osteogenesis.</p><p>Methods: Mouse calvaria-derived osteoblast-like cell line MC3T3-E1 cells (MC) were cultured in αMEM with vitamin C (VC), which augments osteogenic function in osteoblasts, (α+), αMEM without VC (α-), αMEM with VC addition before culture (αVC), DMEM without VC (D-), or DMEM with VC addition before culture (DVC). Cell proliferation, alkaline phosphatase (ALP) activity, cell differentiation marker expression, and bone calcification were compared among the culture conditions.</p><p>Results: MC proliferation was fastest for αVC and slowest for D-. There were notable differences in both ALP activity and differentiation marker expression between αVC and DVC as well as between α+ and αVC. Bone calcification was observed only in the αMEM-based media 3 weeks after the induction of calcification.</p><p>Discussion: Differences in medium type and the presence and freshness of VC all exerted marked effects on MC cell proliferation, ALP activity, cell differentiation, and calcification. Future studies are needed to confirm these findings in other osteoblastic cells and clarify the optimal culture conditions to evaluate bone formation towards the development of international standardized methods.</p>

収録刊行物

詳細情報 詳細情報について

  • CRID
    1390293191190001792
  • DOI
    10.14869/toxpt.49.1.0_p-92s
  • 本文言語コード
    ja
  • データソース種別
    • JaLC
  • 抄録ライセンスフラグ
    使用不可

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