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药理活性微载体释放 TGF-β3 对间充质干细胞体内软骨形成的作用。

The role of pharmacologically active microcarriers releasing TGF-beta3 in cartilage formation in vivo by mesenchymal stem cells.

机构信息

Inserm, U 844, Hôpital Saint-Eloi, 80 avenue Augustin Fliche, Montpellier F-34295, France.

出版信息

Biomaterials. 2010 Sep;31(25):6485-93. doi: 10.1016/j.biomaterials.2010.05.013. Epub 2010 Jun 8.

DOI:10.1016/j.biomaterials.2010.05.013
PMID:20570347
Abstract

Cartilage engineering using mesenchymal stem cells (MSC) will require the use of a scaffold which will act as a support for cell adhesion keeping the cells in the cartilage defect. Optimally, a tissue engineered construct should allow sustained delivery of bioactive factors capable of inducing MSC differentiation into chondrocytes and should be easily injected inside the cartilage lesions to avoid surgical operations. We therefore developed pharmacologically active microcarriers (PAM) made of poly-lactic-co-glycolic acid (PLGA) produced using an oil-in-water (o/w) emulsion method. The microspheres were coated with a biomimetic surface of fibronectin (FN) and engineered to release TGF-beta3 as a chondrogenic differentiation factor. When human MSCs were incubated in vitro with TGF-beta3 releasing FN-coated PAMs in chondrogenic medium, they firmly adhered onto the surface of PAMs rapidly forming cell aggregates. After 3 weeks, strong up-regulation of cartilage-specific markers was observed both at the mRNA and protein level whereas osteogenic or adipogenic genes could not be detected. Importantly, implantation of MSC/TGF-beta3 releasing PAM complexes in SCID mice resulted in the formation of histologically resembling cartilage which stained positive for chondrocyte markers, collagen II and aggrecan. The present study demonstrated that functionalized PLGA-based microparticles can provide an appropriate environment for chondrogenic differentiation of MSCs and should contribute to injectable biomedical device development improving in vivo cartilage engineering.

摘要

使用间充质干细胞(MSC)进行软骨工程将需要使用支架,支架将作为细胞黏附的支撑物,保持细胞在软骨缺陷中。理想情况下,组织工程构建物应允许持续递送能够诱导 MSC 分化为软骨细胞的生物活性因子,并且应易于注射到软骨病变内,以避免手术操作。因此,我们开发了由聚乳酸-共-羟基乙酸(PLGA)制成的药理活性微载体(PAM),使用油包水(o/w)乳液法生产。微球涂有纤维连接蛋白(FN)的仿生表面,并设计为释放 TGF-β3 作为软骨分化因子。当人 MSC 在体外与 TGF-β3 释放的 FN 涂覆的 PAM 在软骨形成培养基中孵育时,它们迅速牢固地黏附在 PAM 的表面上,形成细胞聚集体。3 周后,在 mRNA 和蛋白质水平上均观察到强烈的软骨特异性标志物上调,而未检测到成骨或成脂基因。重要的是,将 MSC/TGF-β3 释放 PAM 复合物植入 SCID 小鼠中导致形成组织学上类似于软骨的结构,其染色阳性的软骨细胞标志物、胶原 II 和聚集蛋白聚糖。本研究表明,功能化的基于 PLGA 的微粒可以为 MSC 的软骨分化提供适当的环境,并且应该有助于可注射生物医学装置的开发,从而改善体内软骨工程。

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