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细胞可降解聚合物-肽水凝胶包封的人骨髓间充质干细胞的性能。

The performance of human mesenchymal stem cells encapsulated in cell-degradable polymer-peptide hydrogels.

机构信息

Department of Chemical and Biological Engineering, University of Colorado, Campus Box 424, Boulder, CO 80309-0424, USA.

出版信息

Biomaterials. 2011 May;32(14):3564-74. doi: 10.1016/j.biomaterials.2011.01.064. Epub 2011 Feb 21.

DOI:10.1016/j.biomaterials.2011.01.064
PMID:21334063
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3085912/
Abstract

Thiol-ene photopolymerization offers a unique platform for the formation of peptide-functionalized poly(ethylene glycol) hydrogels and the encapsulation, culture and differentiation of cells. Specifically, this photoinitiated polymerization scheme occurs at neutral pH and can be controlled both spatially and temporally. Here, we have encapsulated human mesenchymal stem cells (hMSCs) in matrix metalloproteinase (MMP) degradable and cell-adhesive hydrogels using thiol-ene photopolymerization. We find that hMSCs survive equally well in this system, regardless of MMP-degradability. When hMSCs are encapsulated in these cell-degradable hydrogels, they survive and are able to proliferate. In classic hMSC differentiation medias, hMSCs locally remodel their microenvironment and take on characteristic morphologies; hMSCs cultured in growth or osteogenic differentiation media are less round, as measured by elliptical form factor, and are smaller than hMSCs cultured in chondrogenic or adipogenic differentiation media. In addition, hMSCs encapsulated in completely cell-degradable hydrogels and cultured in osteogenic, chondrogenic, or adipogenic differentiation media generally express increased levels of specific differentiation markers as compared to cells in hydrogels that are not cell-degradable. These studies demonstrate the ability to culture and differentiate hMSCs in MMP-degradable hydrogels polymerized via a thiol-ene reaction scheme and that increased cell-mediated hydrogel degradability facilitates directed differentiation of hMSCs.

摘要

硫醇-烯光聚合为形成肽功能化聚(乙二醇)水凝胶以及封装、培养和分化细胞提供了独特的平台。具体而言,这种光引发聚合方案在中性 pH 下发生,并且可以空间和时间控制。在这里,我们使用硫醇-烯光聚合将人骨髓间充质干细胞 (hMSC) 封装在基质金属蛋白酶 (MMP) 可降解和细胞黏附水凝胶中。我们发现 hMSC 在该系统中存活情况相同,与 MMP 降解性无关。当 hMSC 被封装在这些细胞可降解水凝胶中时,它们能够存活并增殖。在经典的 hMSC 分化培养基中,hMSC 局部重塑其微环境并呈现出特征形态;与在成骨或成脂分化培养基中培养的 hMSC 相比,在生长或成软骨分化培养基中培养的 hMSC 不太圆,其椭圆形态因子更小,并且比在成软骨或成脂分化培养基中培养的 hMSC 更小。此外,与不可降解细胞的水凝胶中的细胞相比,封装在完全可降解水凝胶中的 hMSC 并在成骨、软骨或成脂分化培养基中培养通常表现出特定分化标志物的表达水平增加。这些研究证明了在通过硫醇-烯反应方案聚合的 MMP 可降解水凝胶中培养和分化 hMSC 的能力,并且增加的细胞介导的水凝胶降解性促进了 hMSC 的定向分化。

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