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Approaching the compressive modulus of articular cartilage through naturally derived cartilage matrix

机译:通过天然衍生的软骨矩阵接近关节软骨的压缩模量

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Introduction: ECM-based materials are attractive for tissue engineering strategies because they can potentially aid in stem cell recruitment, cell infiltration, and cell differentiation without supplementing with additional biological factors. Although it is a relatively new biomaterial, cartilage ECM has shown potential to be chondroinductive, although in general, hydrogels composed of natural materials are often mechanically inferior to synthetic materials, which may not be ideal for load-bearing tissue applications.13! Therefore, we endeavored to create a hydrogel composed of entirely native cartilage ECM that was mechanically similar to native cartilage tissue and would promote chondrogenesis. Methods: Porcine cartilage was decellularized, solubilized, methacrylated and UV photocrosslinked to create methacrylated solubilized decellularized cartilage (MeSDCC) gels. Methacrylated gelatin (GelMA) was used as a control. Rat bone marrow stem cells were encapsulated in these networks and the constructs were cultured in vitro for 6 weeks, where chondrogenic gene expression, the compressive modulus (linear region of stress-strain curve), swelling, and histology were analyzed. Results and Discussion: One day after crosslinking, the compressive modulus of the 20% MeSDCC gels was 1069.61147.5 kPa (Fig. 1), which is similar to that reported for native cartilage tissue. Figure 1. Compressive Modulus of crosslinked hydrogels after 1 day and 6 weeks of culture. Data reported as mean + standard deviation (n=5); significantly different from 10% GelMA at same time point (p<0.05), #significantly different from 10% MeSDCC at same time point (p<0.05), &p<0.05 for specified comparison, @significantly different from same group at first time point (p<0.05), -not tested. Furthermore, when we compared the stress strain profiles of our 20% MeSDCC gels with native porcine cartilage, the stress strain profile of the 20% MeSDCC gels fell within the 95% confidence interval range of native porcine cartilage until the 20% MeSDCC gels fractured at 7.5% strain. Additionally, MeSDCC gels significantly upregulated chondrogenic genes compared to GelMA at day 1 and supported matrix synthesis as observed with Safrinin-O/Fast Green and H&E staining. Conclusion: Overall, because these gels are approaching the mechanics of native cartilage tissue and because they are supporting matrix synthesis and chondrogenic gene expression, MeSDCC hydrogels may be promising materials for cartilage tissue engineering applications, although future improvements will be necessary for fracture performance. Additionally, future work will evaluate how these gels perform in vivo.
机译:简介:基于ECM的材料对于组织工程策略具有吸引力,因为它们可能有助于干细胞募集,细胞浸润和细胞分化,而无需补充额外的生物因素。虽然它是一种相对较新的生物材料,但软骨ECM显示出潜力是软骨诱导的,尽管通常,由天然材料组成的水凝胶通常是机械差不等的,这可能不是承载组织应用的理想选择.13!因此,我们努力创建一个由完全海豚软骨ECM组成的水凝胶,其机械地类似于天然软骨组织,并会促进软骨发生。方法:猪软骨脱细胞,溶解,甲基丙烯酸和紫外光散,以产生甲基丙烯酸溶化的溶解脱细胞软骨(MESDCC)凝胶。将甲基丙烯酸酯化的明胶(GELMA)用作对照。将大鼠骨髓干细胞包封在这些网络中,并在体外培养构建体6周,其中分析了软骨基因表达,压缩模量(应力 - 应变曲线的线性区域),肿胀和组织学。结果与讨论:交联后一天,20%MESDCC凝胶的压缩模量为1069.61147.5kPa(图1),其类似于本机软骨组织报告的那些。图1. 1天后交联水凝胶的压缩模量和6周的培养物。报告的数据为平均值+标准偏差(n = 5);在同一时间点(P <0.05)同时显着不同于10%的凝胶(P <0.05),与同一时间点(P <0.05),&P <0.05进行指定比较,在第一次相同的组中与相同的组不同(P <0.05), - 测试。此外,当我们将20%MESDCC凝胶与天然猪软骨进行比较时,20%MESDCC凝胶的应力应变曲线下降在95%的天然猪软骨范围内,直至20%MESDCC凝胶裂缝7.5%应变。另外,与白天1天的凝胶凝胶相比,MESDCC凝胶显着上调了软骨内基因,并使用Safrinin-O /快绿色和H&E染色观察到的基质合成。结论:总体而言,由于这些凝胶正在接近天然软骨组织的机制,因为它们支持基质合成和软骨基因表达,因此MESDCC水凝胶可能是软骨组织工程应用的有希望的材料,尽管未来的裂缝性能是必要的。此外,未来的工作将评估这些凝胶如何在体内执行。

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