Choi Dong Hoon, Suhaeri Muhammad, Hwang Mintai P, Kim Ik Hwan, Han Dong Keun, Park Kwideok
Center for Biomaterials, Korea Institute of Science and Technology, Seoul, 136-791, Korea.
Cell Tissue Res. 2014 Sep;357(3):781-92. doi: 10.1007/s00441-014-1898-5. Epub 2014 May 23.
We obtained fibroblast- (FDM) and preosteoblast- (PDM) derived matrices in vitro from their respective cells. Our hypothesis was that these naturally occurring cell-derived matrices (CDMs) would provide a better microenvironment for the multi-lineage differentiation of human mesenchymal stromal cells (hMSCs) than those based on traditional single-protein-based platforms. Cells cultured for 5-6 days were decellularized with detergents and enzymes. The resulting matrices showed a fibrillar surface texture. Under osteogenic conditions, human bone-marrow-derived stromal cells (HS-5) exhibited higher amounts of both mineralized nodule formation and alkaline phosphatase (ALP) expression than those cultured on plastic or gelatin. Osteogenic markers (Col I, osteopontin, and cbfa1) and ALP activity from cells cultured on PDM were notably upregulated at 4 weeks. The use of FDM significantly improved the cellular expression of chondrogenic markers (Sox 9 and Col II), while downregulating that of Col I at 4 weeks. Both CDMs were more effective in inducing cellular synthesis of glycosaminoglycan content than control substrates. We also investigated the effect of matrix surface texture on hMSC (PT-2501) differentiation; soluble matrix (S-matrix)-coated substrates exhibited a localized fibronectin (FN) alignment, whereas natural matrix (N-matrix)-coated substrates preserved the naturally formed FN fibrillar alignment. hMSCs cultured for 4 weeks on N-matrices under osteogenic or chondrogenic conditions deposited a greater amount of calcium and proteoglycan than those cultured on S-matrices as assessed by von Kossa and Safranin O staining. In contrast to the expression levels of lineage-specific markers for cells cultured on gelatin, FN, or S-matrices, those cultured on N-matrices yielded highly upregulated levels. This study demonstrates not only the capacity of CDM for being an effective inductive template for the multi-lineage differentiation of hMSCs, but also the critical biophysical role that the matrix fibrillar texture itself plays on the induction of stem cell differentiation.
我们在体外从成纤维细胞(FDM)和前成骨细胞(PDM)中获取了各自来源的基质。我们的假设是,这些天然存在的细胞衍生基质(CDM)将比基于传统单蛋白平台的基质为人间充质基质细胞(hMSC)的多谱系分化提供更好的微环境。用去污剂和酶对培养5 - 6天的细胞进行脱细胞处理。所得基质呈现出纤维状表面纹理。在成骨条件下,人骨髓来源的基质细胞(HS - 5)比在塑料或明胶上培养的细胞表现出更高的矿化结节形成量和碱性磷酸酶(ALP)表达。在4周时,在PDM上培养的细胞的成骨标志物(I型胶原、骨桥蛋白和cbfa1)和ALP活性显著上调。使用FDM在4周时显著改善了软骨生成标志物(Sox 9和II型胶原)的细胞表达,同时下调了I型胶原的表达。两种CDM在诱导细胞合成糖胺聚糖含量方面都比对照底物更有效。我们还研究了基质表面纹理对hMSC(PT - 2501)分化的影响;可溶性基质(S - 基质)包被的底物呈现局部纤连蛋白(FN)排列,而天然基质(N - 基质)包被的底物保留了天然形成的FN纤维状排列。通过冯·科萨染色和番红O染色评估,在成骨或软骨生成条件下在N - 基质上培养4周的hMSC比在S - 基质上培养的细胞沉积了更多的钙和蛋白聚糖。与在明胶、FN或S - 基质上培养的细胞的谱系特异性标志物表达水平相比,在N - 基质上培养的细胞产生了高度上调的水平。这项研究不仅证明了CDM作为hMSC多谱系分化的有效诱导模板的能力,还证明了基质纤维状纹理本身在诱导干细胞分化中所起的关键生物物理作用。
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