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Phenotypic Stability Matrix Elaboration and Functional Maturation of Nucleus Pulposus Cells Encapsulated in Photocrosslinkable Hyaluronic Acid Hydrogels

机译:光可交联透明质酸水凝胶封装的髓核细胞的表型稳定性基质修饰和功能成熟

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摘要

Degradation of the nucleus pulposus (NP) is an early hallmark of intervertebral disc degeneration. The capacity for endogenous regeneration in the NP is limited due to the low cellularity and poor nutrient supply of this avascular tissue. Towards restoring the NP, a number of biomaterials have been explored for cell delivery. These materials must support the NP cell phenotype while promoting the elaboration of an NP-like extracellular matrix in the shortest possible time. Our previous work with chondrocytes and mesenchymal stem cells demonstrated that hydrogels based on hyaluronic acid (HA) are effective at promoting matrix production and the development of functional material properties. However, this material has not been evaluated in the context of NP cells. Therefore, to test this material for NP regeneration, bovine NP cells were encapsulated in 1% w/vol HA hydrogels at either a low seeding density (20 × 106 cells/ml) or a high seeding density (60 × 106 cells/ml), and constructs were cultured over an 8 week period. These engineered NP cell-laden HA hydrogels showed functional matrix accumulation, with increasing matrix content and mechanical properties with time in culture at both seeding densities. Furthermore, encapsulated cells showed NP-specific gene expression profiles that were significantly higher than expanded NP cells prior to encapsulation, suggesting a restoration of phenotype. Interestingly, these levels were higher at the lower seeding density compared to the higher seeding density. These findings support the use of HA-based hydrogels for NP tissue engineering and cellular therapies directed at restoration or replacement of the endogenous NP.
机译:髓核(NP)的退化是椎间盘退变的早期标志。 NP中内源性再生的能力由于该无血管组织的低细胞性和不良的营养供应而受到限制。为了恢复NP,已经探索了许多生物材料用于细胞递送。这些材料必须支持NP细胞表型,同时在最短的时间内促进NP样细胞外基质的形成。我们先前对软骨细胞和间充质干细胞的研究表明,基于透明质酸(HA)的水凝胶可有效促进基质的产生和功能材料性能的发展。但是,该材料尚未在NP细胞的背景下进行评估。因此,为了测试这种材料的NP再生,将牛NP细胞以低接种密度(20×10 6 细胞/ ml)或高接种密度封装在1%w / vol HA水凝胶中(60×10 6 细胞/ ml),并在8周内培养构建体。在两种播种密度下,这些经过工程处理的富含NP细胞的HA水凝胶均显示出功能性基质蓄积,随着时间的流逝,基质含量和机械性能均随时间增加。此外,被囊化的细胞显示出NP特异性基因表达谱,其显着高于被囊化之前的扩增的NP细胞,表明表型得以恢复。有趣的是,与较高的播种密度相比,这些浓度在较低的播种密度下较高。这些发现支持基于HA的水凝胶用于NP组织工程和针对内源性NP的修复的细胞疗法。

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