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用于组织工程的差异脱矿松质骨支架与人骨髓基质细胞联合的体外和体内评价

In vitro and in vivo evaluation of differentially demineralized cancellous bone scaffolds combined with human bone marrow stromal cells for tissue engineering.

作者信息

Mauney Joshua R, Jaquiéry Claude, Volloch Vladimir, Heberer Michael, Martin Ivan, Kaplan David L

机构信息

Department of Biomedical Engineering, Tufts University, Biotechnology Center, 4 Colby Street, Medford, MA 02155, USA.

出版信息

Biomaterials. 2005 Jun;26(16):3173-85. doi: 10.1016/j.biomaterials.2004.08.020.

Abstract

Mineralized and partially or fully demineralized biomaterials derived from bovine bone matrix were evaluated for their ability to support human bone marrow stromal cell (BMSC) osteogenic differentiation in vitro and bone-forming capacity in vivo in order to assess their potential use in clinical tissue-engineering strategies. BMSCs were either seeded on bone-derived scaffolds and cocultured in direct cell-to-scaffold contact, allowing for the exposure of soluble and insoluble matrix-incorporated factors, or cocultured with the scaffold preparations in a transwell system, exposing them to soluble matrix-incorporated factors alone. Osteoblast-related markers, alkaline phosphatase (ALP) activity and bone sialoprotein (BSP) and osteopontin (OP) mRNA expression were evaluated in BMSCs following 14 days of cocultivation in both systems. The data demonstrate that BMSCs from some donors express significantly higher levels of all osteoblast-related markers following cocultivation in direct cell-to-scaffold contact with mineralized scaffolds in comparison to fully demineralized preparations, while BMSCs from other donors display no significant differences in response to various scaffold preparations. In contrast, BMSCs cocultured independently with soluble matrix-incorporated factors derived from each scaffold preparation displayed significantly lower levels of ALP activity and BSP mRNA expression in comparison to untreated controls, while no significant differences were observed in marker levels between cells cocultured similarly with different biomaterial preparations. In addition, BMSCs were seeded directly on mineralized and partially or fully demineralized biomaterials and implanted in subcutaneous sites of athymic mice for 8 weeks to evaluate their in vivo bone-forming capacity. The ex vivo incorporation of BMSCs into all bone-derived scaffold preparations substantially increased the mean extent and frequency of samples containing de novo bone formation over similar nonseeded controls, as determined by histological and histomorphometrical analysis. No statistically significant differences were observed in the extent or frequency of bone formation between various scaffold preparations seeded with BMSCs from different donors. These results demonstrate that the in vivo osteoinductivity of bone-derived scaffolds can be modulated by ex vivo incorporated BMSCs and the extent of scaffold demineralization plays a significant role in influencing in vitro osteogenic differentiation of BMSCs depending on the coculture system and BMSC donor.

摘要

为了评估从牛骨基质中提取的矿化及部分或完全脱矿的生物材料在临床组织工程策略中的潜在应用,对其在体外支持人骨髓基质细胞(BMSC)成骨分化的能力以及在体内的骨形成能力进行了评估。将BMSC接种在骨源支架上,以细胞与支架直接接触的方式共培养,使细胞能够接触可溶性和不可溶性的基质结合因子;或者在transwell系统中与支架制剂共培养,使细胞仅接触可溶性基质结合因子。在两种系统中共培养14天后评估BMSC中与成骨细胞相关的标志物、碱性磷酸酶(ALP)活性以及骨唾液蛋白(BSP)和骨桥蛋白(OP)mRNA的表达。数据表明,与完全脱矿的制剂相比,在与矿化支架进行细胞与支架直接接触的共培养后,来自某些供体的BMSC表达的所有与成骨细胞相关的标志物水平显著更高,而来自其他供体的BMSC对各种支架制剂没有显著差异。相反,与未处理的对照相比,与每种支架制剂中可溶性基质结合因子独立共培养的BMSC显示出显著更低的ALP活性和BSP mRNA表达水平,而与不同生物材料制剂进行类似共培养的细胞之间的标志物水平没有显著差异。此外,将BMSC直接接种在矿化及部分或完全脱矿的生物材料上,并植入无胸腺小鼠的皮下部位8周,以评估其体内骨形成能力。通过组织学和组织形态计量学分析确定,与类似的未接种对照相比,BMSC在所有骨源支架制剂中的体外掺入显著增加了含有新生骨形成的样本的平均范围和频率。在接种来自不同供体的BMSC的各种支架制剂之间,未观察到骨形成范围或频率的统计学显著差异。这些结果表明,骨源支架的体内骨诱导性可通过体外掺入的BMSC进行调节,并且支架脱矿程度在影响BMSC的体外成骨分化方面起着重要作用,这取决于共培养系统和BMSC供体。

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