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Reversible mitotic and metabolic inhibition following the encapsulation of fibroblasts in alginate hydrogels.

机译:在藻酸盐水凝胶中包裹成纤维细胞后,可逆的有丝分裂和代谢抑制作用。

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摘要

Limiting cell proliferation without reducing cell viability for in vivo tissue engineering applications is important in co-culture applications where the growth of one cell type must be inhibited to prevent overgrowth of the scaffold at the expense of another cell type. Also, it is vital for maintaining viability of cells in large constructs before vascularisation occurs. In this study we have shown by means of the Thiazolyl blue (MTT) assay and immuno-staining for proliferating cell nuclear antigen (PCNA) that encapsulating fibroblasts in 2% and 5%w/v calcium-alginate at a density of 7.5 x 10(5)cells/ml as uniformly dispersed entities, enabled cells to maintain viability and caused a reversible mitotic inhibition. Alginate encapsulation also caused reversible metabolic inhibition as demonstrated by the MTT assay and fluorescent staining for mitochondrial membrane potential. Histological evaluation of the alginate constructs containing fibroblasts showed that mitotic and metabolic inhibition was possibly due to cell isolation during the first five weeks of culture. The alginate scaffold degraded with time releasing encapsulated fibroblasts. Upon implantation to a wound site this should ensure that encapsulated cells are able to replace the damaged tissue after sufficient proliferation of the co-cultured cell type or sufficient vascularisation of the construct.
机译:对于体内组织工程应用而言,在不降低细胞生存力的情况下限制细胞增殖在共培养应用中非常重要,在共培养应用中,必须抑制一种细胞类型的生长以防止支架过度生长,而牺牲另一种细胞类型。同样,对于在发生血管化之前在大型构建物中维持细胞活力至关重要。在这项研究中,我们已经证明了通过噻唑蓝(MTT)测定和免疫染色的增殖细胞核抗原(PCNA),可以将成纤维细胞封装在2%和5%w / v海藻酸钙中,密度为7.5 x 10 (5)cells / ml作为均匀分散的实体,使细胞保持活力并引起可逆的有丝分裂抑制。如MTT测定和线粒体膜电位的荧光染色所证实的,藻酸盐包封还引起可逆的代谢抑制。对含有成纤维细胞的藻酸盐构建物的组织学评估表明,有丝分裂和代谢抑制作用可能是由于在培养的前五周内细胞分离所致。藻酸盐支架随时间降解,释放封装的成纤维细胞。在植入伤口部位后,这应确保在共培养的细胞类型充分增殖或构建体充分血管化后,包囊细胞能够替代受损组织。

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