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Macrophage Adhesion on Gelatin-Based Interpenetrating Networks Grafted with PEGylated RGD.

机译:巨噬细胞在基于PEG的RGD接枝的基于明胶的互穿网络上的粘附。

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摘要

Human blood-derived macrophage adhesion on interpenetrating networks (IPNs) composed of PEGylated RGD-modified gelatin and poly(ethylene glycol) diacrylate was studied. The interaction between biomaterial immobilized with biofunctional peptides such as RGD and macrophages is central in the design of tissue-engineering scaffolds. PEGylated RGD-modified gelatin was synthesized via several steps involving PEG derivations and characterized by high-performance liquid chromatography, mass spectroscopy, gel permeation chromatography, and the trinitrobenzenesulfonic acid method. IPNs containing modified or unmodified gelatin were cultured with human macrophages and monitored at 2, 24, 96, and 168 h. At each time point, IPNs containing gelatin modified with PEGylated RGD showed a comparable adherent macrophage density as tissue culture polystyrene and a significantly higher cell density than other IPN formulations containing unmodified gelatin or gelatin modified with PEGylated triglycine. Although surface-immobilized RGD can serve to mediate the adhesion of different cell types on the biomaterial surface, the interaction of RGD with immune/inflammatory cells such as macrophages should also be considered when assessing the potential host response of tissue-engineering scaffolds.
机译:研究了人类血液来源的巨噬细胞在由PEG化RGD改性的明胶和聚乙二醇二丙烯酸酯组成的互穿网络(IPN)上的粘附。固定有生物功能肽(例如RGD)的生物材料与巨噬细胞之间的相互作用在组织工程支架的设计中至关重要。 PEG化的RGD修饰的明胶是通过涉及PEG衍生的多个步骤合成的,并通过高效液相色谱,质谱,凝胶渗透色谱和三硝基苯磺酸方法进行了表征。用人类巨噬细胞培养含有修饰或未修饰明胶的IPN,并在2、24、96和168小时进行监测。在每个时间点,含有经聚乙二醇化RGD修饰的明胶的IPN的粘附巨噬细胞密度与组织培养聚苯乙烯相当,并且细胞密度明显高于其他未经修饰的明胶或经聚乙二醇化三甘氨酸修饰的明胶的IPN制剂。尽管表面固定的RGD可以用来介导生物材料表面上不同细胞类型的粘附,但在评估组织工程支架的潜在宿主反应时,也应考虑RGD与免疫/炎症细胞(例如巨噬细胞)的相互作用。

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