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Novel methodology based on biomimetic superhydrophobic substrates to immobilize cells and proteins in hydrogel spheres for applications in bone regeneration

机译:基于仿生超疏水底物的新型方法,可将细胞和蛋白质固定在水凝胶球体中,用于骨骼再生

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摘要

Cell-based therapies for regenerative medicine have been characterized by the low retention and integration of injected cells into host structures. Cell immobilization in hydrogels for target cell delivery has been developed to circumvent this issue. In this work mesenchymal stem cells isolated from Wistar rats bone marrow (rMSCs) were immobilized in alginate beads fabricated using an innovative approach involving the gellification of the liquid precursor droplets onto biomimetic superhydrophobic surfaces without the need of any precipitation bath. The process occurred in mild conditions preventing the loss of cell viability. Furthermore, fibronectin (FN) was also immobilized inside alginate beads with high efficiency in order to mimic the composition of the extracellular matrix. This process occurred in a very fast way (around 5 min), at room temperature, without aggressive mechanical strengths or particle aggregation. The methodology employed allowed the production of alginate beads exhibiting a homogenous rMSCs and FN distribution. Encapsulated rMSCs remained viable and were released from the alginate for more than 20 days. In vivo assays were also performed, by implanting these particles in a calvarial bone defect to evaluate their potential for bone tissue regeneration. Microcomputed tomography and histological analysis results showed that this hybrid system accelerated bone regeneration process. The methodology employed had a dual role by preventing cell and FN loss and avoiding any contamination of the beads or exchange of molecules with the surrounding environment. In principle, the method used for cell encapsulation could be extended to other systems aimed to be used in tissue regeneration strategies.
机译:再生医学的基于细胞的疗法的特点是注射细胞的滞留率低和整合到宿主结构中。已经开发出将水凝胶中的细胞固定化以用于靶细胞递送来解决这个问题。在这项工作中,将从Wistar大鼠骨髓(rMSCs)分离的间充质干细胞固定在藻酸盐珠中,藻酸盐珠采用创新方法制备,涉及将液态前体液滴胶凝到仿生超疏水表面上,而无需任何沉淀浴。该过程发生在温和的条件下,阻止了细胞活力的丧失。此外,为了模拟细胞外基质的组成,纤连蛋白(FN)也被高效地固定在藻酸盐珠内。该过程在室温下以非常快的方式(约5分钟)发生,没有强烈的机械强度或颗粒聚集。所使用的方法允许藻酸盐珠粒的产生,所述藻酸盐珠粒具有均匀的rMSC和FN分布。封装的rMSC仍然可以存活,并且从藻酸盐中释放超过20天。通过将这些颗粒植入颅骨缺损中以评估其在骨组织再生中的潜力,还进行了体内测定。微计算机断层扫描和组织学分析结果表明,该混合系统加速了骨再生过程。所采用的方法具有双重作用,可以防止细胞和FN的损失,避免珠子的污染或与周围环境的分子交换。原则上,用于细胞封装的方法可以扩展到旨在用于组织再生策略的其他系统。

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