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Bioactive nanofibers enable the identification of thrombospondin 2 as a key player in enamel regeneration

机译:具有生物活性的纳米纤维可将血小板反应蛋白2鉴定为搪瓷再生的关键参与者

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摘要

Tissue regeneration and development involves highly synchronized signals both between cells and with the extracellular environment. Biomaterials can be tuned to mimic specific biological signals and control cell response(s). As a result, these materials can be used as tools to elucidate cell signaling pathways and candidate molecules involved with cellular processes. In this work, we explore enamel-forming cells, ameloblasts, which have a limited regenerative capacity. By exposing undifferentiated cells to a self-assembling matrix bearing RGDS epitopes, we elicited a regenerative signal at will that subsequently led to the identification of thrombospondin 2 (TSP2), an extracellular matrix protein that has not been previously recognized as a key player in enamel development and regeneration. Targeted disruption of the thrombospondin 2 gene (Thbs2) resulted in enamel formation with a disordered architecture that was highly susceptible to wear compared to their wild-type counterparts. To test the regenerative capacity, we injected the bioactive matrix into the enamel organ and discovered that the enamel organic epithelial cells in TSP-null mice failed to polarize on the surface of the artificial matrix, greatly reducing integrin β1 and Notch1 expression levels, which represent signaling pathways known to be associated with TSP2. These results suggest TSP2 plays an important role in regulating cell-matrix interactions during enamel formation. Exploiting the signaling pathways activated by biomaterials can provide insight into native signaling mechanisms crucial for tooth development and cell-based strategies for enamel regeneration.
机译:组织再生和发育涉及细胞之间以及细胞外环境的高度同步信号。可以调整生物材料以模仿特定的生物信号并控制细胞反应。结果,这些材料可以用作阐明细胞信号传导途径和与细胞过程有关的候选分子的工具。在这项工作中,我们探索搪瓷形成细胞,成釉细胞,其再生能力有限。通过将未分化的细胞暴露于带有RGDS表位的自组装基质中,我们随意产生了再生信号,随后导致鉴定出血小板反应蛋白2(TSP2),这是一种以前未被认为是牙釉质关键参与者的细胞外基质蛋白。发展和再生。血小板反应蛋白2基因(Thbs2)的定向破坏导致牙釉质形成,其结构紊乱,与野生型对应物相比,极易磨损。为了测试其再生能力,我们将生物活性基质注入牙釉质器官,并发现TSP无效小鼠的牙釉质有机上皮细胞未能在人工基质表面极化,从而大大降低了整联蛋白β1和Notch1的表达水平。已知与TSP2相关的信号通路。这些结果表明TSP2在搪瓷形成过程中调节细胞-基质相互作用中起着重要作用。利用生物材料激活的信号通路可以提供对牙齿发育至关重要的天然信号传导机制以及牙釉质再生基于细胞的策略的洞察力。

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