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明胶-纤维蛋白原胶原纤维蛋白冷冻凝胶真皮基质在创面修复中的应用:制备、优化及体外研究。

Gelatin-fibrinogen cryogel dermal matrices for wound repair: preparation, optimisation and in vitro study.

机构信息

Protista Biotechnology AB, IDEON, SE 223 70,Lund, Sweden.

出版信息

Biomaterials. 2010 Jan;31(1):67-76. doi: 10.1016/j.biomaterials.2009.09.029. Epub 2009 Sep 27.

DOI:10.1016/j.biomaterials.2009.09.029
PMID:19783036
Abstract

Macroporous sponge-like gelatin-fibrinogen (Gl-Fg) scaffolds cross-linked with different concentrations (0.05-0.5%) of glutaraldehyde (GA) were produced using cryogelation technology, which allows for the preparation of highly porous scaffolds without compromising their mechanical properties, and is a more cost-efficient process than freeze-drying. The produced Gl-Fg-GA(X) scaffolds had a uniform interconnected open porous structure with a porosity of up to 90-92% and a pore size distribution of 10-120 microm. All of the obtained cryogels were elastic and mechanically stable, except for the Gl-Fg-GA(0.05) scaffolds. Swelling kinetics and degradation rate, but not the porous structure of the cryogels, were strongly dependent on the degree of cross-linking. A ten-fold increase in the degree of cross-linking resulted in an almost 80-fold decrease in the rate of degradation in a solution of protease. Cryogels were seeded with primary dermal fibroblasts and the densities observed on the surface, plus the expression levels of collagen types I and III observed 5 days post-seeding, were similar to those observed on a control dermal substitute material, Integra. Fibroblast proliferation and migration within the scaffolds were relative to the GA content. Glucose consumption rate was 3-fold higher on Gl-Fg-GA(0.1) than on Gl-Fg-GA(0.5) cryogels 10 days post-seeding. An enhanced cell motility on cryogels with reducing GA crosslinking was obtained after long time culture. Particularly marked cell infiltration was seen in gels using 0.1% GA as a crosslinker. The scaffold started to disintegrate after 42 days of in vitro culturing. The described in vitro studies demonstrated good potential of Gl-Fg-GA(0.1) scaffolds as matrices for wound healing.

摘要

使用冷冻凝胶技术制备了不同戊二醛(GA)交联浓度(0.05-0.5%)的大孔海绵状明胶-纤维蛋白原(Gl-Fg)支架,这种技术可以在不影响其机械性能的情况下制备高度多孔的支架,而且比冷冻干燥更具成本效益。所制备的 Gl-Fg-GA(X)支架具有均匀的互连开放式多孔结构,孔隙率高达 90-92%,孔径分布为 10-120μm。所有获得的冷冻凝胶都是弹性和机械稳定的,除了 Gl-Fg-GA(0.05)支架。凝胶的溶胀动力学和降解速率,但不是多孔结构,强烈依赖于交联度。交联度增加十倍会导致在蛋白酶溶液中的降解速率几乎降低 80 倍。将原代真皮成纤维细胞接种到冷冻凝胶上,在接种后 5 天观察到的表面密度以及 I 型和 III 型胶原的表达水平,与对照真皮替代物 Integra 相似。细胞在支架内的增殖和迁移与 GA 含量有关。与 Gl-Fg-GA(0.5)冷冻凝胶相比,Gl-Fg-GA(0.1)冷冻凝胶上的葡萄糖消耗率在接种后 10 天增加了 3 倍。经过长时间培养,在 GA 交联减少的冷冻凝胶上获得了增强的细胞迁移能力。在使用 0.1% GA 作为交联剂的凝胶中观察到特别明显的细胞浸润。在体外培养 42 天后,支架开始分解。所述体外研究表明,Gl-Fg-GA(0.1)支架作为伤口愈合的基质具有良好的潜力。

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