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在承重小梁形状记忆合金支架上骨髓间充质干细胞的增殖和分化。

Mesenchymal stem cell proliferation and differentiation on load-bearing trabecular Nitinol scaffolds.

机构信息

Department of Materials Science and Engineering, Technion-Israel Institute of Technology, Haifa 32000, Israel.

出版信息

Acta Biomater. 2013 Sep;9(9):8440-8. doi: 10.1016/j.actbio.2013.05.030. Epub 2013 Jun 5.

DOI:10.1016/j.actbio.2013.05.030
PMID:23747323
Abstract

Bone tissue regeneration in load-bearing regions of the body requires high-strength porous scaffolds capable of supporting angiogenesis and osteogenesis. 70% porous Nitinol (NiTi) scaffolds with a regular 3-D architecture resembling trabecular bone were produced from Ni foams using an original reactive vapor infiltration technique. The "trabecular Nitinol" scaffolds possessed a high compressive strength of 79 MPa and high permeability of 6.9×10(-6) cm2. The scaffolds were further modified to produce a near Ni-free surface layer and evaluated in terms of Ni ion release and human mesenchymal stem cell (hMSC) proliferation (AlamarBlue), differentiation (alkaline phosphatase activity, ALP) and mineralization (Alizarin Red S staining). Scanning electron microscopy was employed to qualitatively corroborate the results. hMSCs were able to adhere and proliferate on both as-produced and surface-modified trabecular NiTi scaffolds, to acquire an osteoblastic phenotype and produce a mineralized extracellular matrix. Both ALP activity and mineralization were increased on porous scaffolds compared to control polystyrene plates. Experiments in a model coculture system of microvascular endothelial cells and hMSCs demonstrated the formation of prevascular structures in trabecular NiTi scaffolds. These data suggest that load-bearing trabecular Nitinol scaffolds could be effective in regenerating damaged or lost bone tissue.

摘要

在承重区域的骨组织再生需要高强度的多孔支架,能够支持血管生成和成骨。采用原创的反应性气相渗透技术,从镍泡沫中制备出具有类似于小梁骨的规则 3-D 结构的 70%多孔 Nitinol(NiTi)支架。“小梁 Nitinol”支架具有 79 MPa 的高抗压强度和 6.9×10(-6)cm2 的高渗透性。进一步对支架进行改性,生成近无 Ni 表面层,并评价 Ni 离子释放和人骨髓间充质干细胞(hMSC)增殖(AlamarBlue)、分化(碱性磷酸酶活性,ALP)和矿化(茜素红 S 染色)。采用扫描电子显微镜对结果进行定性验证。hMSCs 能够在原始和表面改性的小梁 NiTi 支架上黏附和增殖,获得成骨表型并产生矿化细胞外基质。与对照聚苯乙烯板相比,多孔支架上的 ALP 活性和矿化均增加。在微血管内皮细胞和 hMSCs 的模型共培养系统中进行的实验表明,小梁 Nitinol 支架中形成了预血管结构。这些数据表明,承重小梁 Nitinol 支架可有效再生受损或丢失的骨组织。

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