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猪间充质基质细胞的特性及其在长期培养中的增殖和成骨潜力

Characterization of porcine mesenchymal stromal cells and their proliferative and osteogenic potential in long-term culture.

作者信息

Zimmermann Corinna E, Mackens-Kiani Lars, Acil Yahya, Terheyden Hendrik

机构信息

Department of Craniomaxillofacial Surgery, University Hospital Schleswig-Holstein, Campus Kiel, Arnold-Heller-Strasse 3, 24105 Kiel, Germany.

University of Lübeck, Ratzeburger Allee 160, 23562 Lübeck, Germany.

出版信息

J Stem Cells Regen Med. 2021 Dec 30;17(2):49-55. doi: 10.46582/jsrm.1702008. eCollection 2021.

Abstract

Porcine mesenchymal stromal cells (pMSCs) are considered a valuable research model for bone tissue engineering, which requires adequate amounts of viable cells with sufficient potential for osteogenic differentiation. For isolation and expansion of these cells through long-term culture, appropriate culture conditions are needed. To study the effect of extended cultivation on pMSC proliferation and differentiation potential using different osteogenic and adipogenic induction media. pMSCs were isolated from the bone marrow of adult Göttingen minipigs, cultured, expanded to passage 20 (~160 days) and characterized by their expression of cell surface markers (wCD44, CD45, CD90, SWC9, fibronectin), alkaline phosphatase (ALP), and osteocalcin and their potential for osteogenic and adipogenic differentiation using different induction media. pMSCs retained their capacity for proliferation and osteogenic differentiation, and the number of CD90-positive cells increased significantly over more than 60 population doublings. CD90 expression in uninduced cells correlated strongly with ALP expression following osteogenic induction. Medium enriched with calcium yielded a stronger osteogenic response. The selection of CD90-positive MSCs and adequate levels of calcium seem to enhance the osteogenic phenotype for bone tissue engineering.

摘要

猪间充质基质细胞(pMSCs)被认为是骨组织工程的一种有价值的研究模型,该模型需要足够数量的具有充分成骨分化潜力的活细胞。为了通过长期培养分离和扩增这些细胞,需要合适的培养条件。为了使用不同的成骨和脂肪生成诱导培养基研究延长培养对pMSC增殖和分化潜力的影响。从成年哥廷根小型猪的骨髓中分离pMSCs,进行培养,扩增至第20代(约160天),并通过细胞表面标志物(wCD44、CD45、CD90、SWC9、纤连蛋白)、碱性磷酸酶(ALP)和骨钙素的表达以及使用不同诱导培养基进行成骨和脂肪生成分化的潜力对其进行表征。pMSCs保留了增殖和成骨分化的能力,并且在超过60次群体倍增后,CD90阳性细胞的数量显著增加。未诱导细胞中的CD90表达与成骨诱导后的ALP表达密切相关。富含钙的培养基产生更强的成骨反应。选择CD90阳性的MSCs和适当水平的钙似乎可以增强骨组织工程的成骨表型。

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