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细胞黏附及对含磷酸三钙和脯氨醇的光固化可降解骨黏合剂的反应。

Cell attachment and response to photocured, degradable bone adhesives containing tricalcium phosphate and purmorphamine.

机构信息

Biomaterials and Tissue Engineering, UCL Eastman Dental Institute, 256 Gray's Inn Road, London WC1X 8LD, UK.

出版信息

Acta Biomater. 2011 Jun;7(6):2672-7. doi: 10.1016/j.actbio.2011.02.033. Epub 2011 Feb 25.

DOI:10.1016/j.actbio.2011.02.033
PMID:21354477
Abstract

The aim of this study was to quantify and provide evidence as to how addition of tricalcium phosphate (β-TCP) and the Hedgehog agonist purmorphamine to a degradable bone adhesive affects cell attachment/proliferation and Hedgehog pathway activation. Fourier transform infrared spectroscopy demonstrated that high levels (75 wt.%) of β-TCP addition reduced the photocure rate of the chosen poly(propylene glycol-co-lactide) dimethacrylate (PPLM) bone adhesive, but this problem was overcome by increased light exposure. In phosphate-buffered saline the total surface mass loss of set 15 mm diameter PPLM films was ∼3.2 mg in 12 weeks, irrespective of thickness (200 or 400 μm) or β-TCP level (50 or 75 wt.%). With 400 μm samples there was additional bulk material loss. Proliferation of pre-osteoblast cells (MC3T3-E1) on the set adhesive surfaces was enhanced by decreased sample thickness or filler content increase. Degradation evidence suggested that both effects were due to reduced acidic polymeric degradation products. Activation of the Hedgehog pathway was quantified by measuring Gli expression in Light II reporter cells. The 0.01 and 0.1 wt.% purmorphamine in composite discs (400 μm, 75 wt.% β-TCP) enhanced Gli expression of attached cells 2- and 5-fold, respectively, without influencing their number. Pre-storage of the composite samples in culture medium had no detrimental effect on this response. Furthermore, sample storage medium gave no enhanced Gli expression in cells on tissue culture plastic. This suggests drug release levels were very low. Purmorphamine and β-TCP incorporation in PPLM adhesives might, therefore, provide prolonged enhancement of in vivo bone repair without systemic drug side-effects.

摘要

本研究旨在定量评估并提供证据,证明在可降解骨胶中添加磷酸三钙(β-TCP)和 Hedgehog 激动剂 Purmorphamine 对细胞附着/增殖和 Hedgehog 通路激活的影响。傅里叶变换红外光谱表明,高浓度(75wt.%)β-TCP 的添加降低了所选聚(丙二醇-co-乳酸)二甲基丙烯酸酯(PPLM)骨胶的光固化速率,但通过增加光暴露可以解决这个问题。在磷酸盐缓冲盐水中,设定的 15mm 直径 PPLM 薄膜的总表面质量损失在 12 周内约为 3.2mg,与厚度(200 或 400μm)或β-TCP 水平(50 或 75wt.%)无关。对于 400μm 样品,还有额外的体相材料损失。前成骨细胞(MC3T3-E1)在已凝固的胶黏剂表面的增殖通过降低样本厚度或增加填充剂含量而增强。降解证据表明,这两种效应都归因于酸性聚合物降解产物的减少。通过测量 Light II 报告细胞中的 Gli 表达来定量 Hedgehog 通路的激活。复合盘中 0.01wt.%和 0.1wt.%的 Purmorphamine(400μm,75wt.%β-TCP)分别将附着细胞的 Gli 表达增强了 2 倍和 5 倍,而不影响细胞数量。在培养中预先储存复合样本对该反应没有不利影响。此外,样品储存介质在组织培养塑料上的细胞中没有增强 Gli 表达。这表明药物释放水平非常低。因此,将 Purmorphamine 和β-TCP 掺入 PPLM 胶黏剂中可能会在体内骨修复中提供持续的增强作用,而不会产生系统性药物副作用。

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