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在 PEG 微球和 TGF-β3 的存在下,人 MSC 聚集物中软骨细胞表达谱的变化。

Changes of chondrocyte expression profiles in human MSC aggregates in the presence of PEG microspheres and TGF-β3.

机构信息

Department of Orthopaedic Surgery, Washington University School of Medicine, 660 South Euclid Avenue, St Louis, MO 63110, USA.

出版信息

Biomaterials. 2011 Nov;32(33):8436-45. doi: 10.1016/j.biomaterials.2011.07.056. Epub 2011 Aug 4.

DOI:10.1016/j.biomaterials.2011.07.056
PMID:21820171
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3176960/
Abstract

Biomaterial microparticles are commonly utilized as growth factor delivery vehicles to induce chondrogenic differentiation of mesenchymal stem/stromal cells (MSCs). To address whether the presence of microparticles could themselves affect differentiation of MSCs, a 3D co-aggregate system was developed containing an equal volume of human primary bone marrow-derived MSCs and non-degradable RGD-conjugated poly(ethylene glycol) microspheres (PEG-μs). Following TGF-β3 induction, differences in cell phenotype, gene expression and protein localization patterns were found when compared to MSC aggregate cultures devoid of PEG-μs. An outer fibrous layer always found in differentiated MSC aggregate cultures was not formed in the presence of PEG-μs. Type II collagen protein was synthesized by cells in both culture systems, although increased levels of the long (embryonic) procollagen isoforms were found in MSC/PEG-μs aggregates. Ubiquitous deposition of type I and type X collagen proteins was found in MSC/PEG-μs cultures while the expression patterns of these collagens was restricted to specific areas in MSC aggregates. These findings show that MSCs respond differently to TGF-β3 when in a PEG-μs environment due to effects of cell dilution, altered growth factor diffusion and/or cellular interactions with the microspheres. Although not all of the expression patterns pointed toward improved chondrogenic differentiation in the MSC/PEG-μs cultures, the surprisingly large impact of the microparticles themselves should be considered when designing drug delivery/scaffold strategies.

摘要

生物材料微粒通常被用作生长因子的递送载体,以诱导间充质干细胞/基质细胞(MSCs)的软骨分化。为了研究微粒本身是否会影响 MSCs 的分化,开发了一种 3D 共聚集系统,其中包含等量的人原代骨髓来源的 MSCs 和不可降解的 RGD 缀合聚乙二醇微球(PEG-μs)。与不含 PEG-μs 的 MSC 聚集培养物相比,在 TGF-β3 诱导后,发现细胞表型、基因表达和蛋白质定位模式存在差异。在外源性 TGF-β3 诱导后,在含有 PEG-μs 的情况下,未形成总是在分化的 MSC 聚集培养物中发现的外层纤维状层。两种培养系统中的细胞均合成 II 型胶原蛋白,尽管 MSC/PEG-μs 聚集物中发现了较高水平的长(胚胎)前胶原同工型。在 MSC/PEG-μs 培养物中发现了普遍存在的 I 型和 X 型胶原蛋白沉积,而这些胶原蛋白的表达模式仅限于 MSC 聚集物的特定区域。这些发现表明,由于细胞稀释、生长因子扩散改变和/或细胞与微球的相互作用,MSCs 在 PEG-μs 环境中对 TGF-β3 的反应不同。尽管并非所有的表达模式都表明 MSC/PEG-μs 培养物中的软骨分化得到了改善,但在设计药物输送/支架策略时,应考虑到微粒本身的巨大影响。

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