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中性粒细胞介导的分段聚氨酯降解

Neutrophil-mediated degradation of segmented polyurethanes.

作者信息

Labow R S, Erfle D J, Santerre J P

机构信息

Cardiovascular Devices Division, University of Ottawa Heart Institute, Ottawa Civic Hospital, ON, Canada.

出版信息

Biomaterials. 1995 Jan;16(1):51-9. doi: 10.1016/0142-9612(95)91096-h.

DOI:10.1016/0142-9612(95)91096-h
PMID:7718693
Abstract

The biostability of polyurethanes was evaluated using a human neutrophil cell culture. The polymers were synthesized with 14C radiolabelled components incorporated into the polyurethane chain and the amount of radiolabel released during exposure to cells and medium was used as a marker for material degradation. The effect of diisocyanate, soft segment and chain extender chemistry on the susceptibility of polymer degradation was examined. All polymers showed a release of material into the tissue culture medium which was unrelated to the cells. A significant cell-dependent release of radiolabel-containing material was found from one of the polymers (a polyester urea-urethane, TDI/PCL/ED) which increased linearly up to 96 h. The polyether-containing polyurethanes showed no significant cell-mediated degradation under similar conditions as measured by radiolabel release. Scanning electron microscopy (SEM) showed that the cells adhered to the different polyurethanes. However, no effect of neutrophils on polymer structure could be detected by this technique. The cellular response to each polymer was evaluated by measuring release of elastase-like activity (ELA) into the tissue culture media. After 24h TDI/PCL/ED showed the highest levels of ELA in the tissue culture medium. When TDI/PCL/ED was incubated with commercial elastase in vitro, a significant release of radiolabel was found which was comparable to the amount of radiolabelled material released from this polymer in contact with the neutrophils in culture. No significant amount of radiolabel was released from the corresponding polyether material (TDI/PTMO/ED) under similar conditions.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

使用人类中性粒细胞培养物评估聚氨酯的生物稳定性。这些聚合物是用掺入聚氨酯链中的14C放射性标记成分合成的,在细胞和培养基暴露期间释放的放射性标记量用作材料降解的标志物。研究了二异氰酸酯、软段和扩链剂化学性质对聚合物降解敏感性的影响。所有聚合物都向组织培养基中释放了与细胞无关的物质。从一种聚合物(聚酯脲聚氨酯,TDI/PCL/ED)中发现了显著的依赖细胞的含放射性标记物质的释放,这种释放在96小时内呈线性增加。通过放射性标记释放测量,在类似条件下,含聚醚的聚氨酯未显示出明显的细胞介导降解。扫描电子显微镜(SEM)显示细胞附着在不同的聚氨酯上。然而,通过该技术未检测到中性粒细胞对聚合物结构的影响。通过测量组织培养基中类弹性蛋白酶活性(ELA)的释放来评估细胞对每种聚合物的反应。24小时后,TDI/PCL/ED在组织培养基中显示出最高水平的ELA。当TDI/PCL/ED在体外与商业弹性蛋白酶孵育时,发现有显著的放射性标记释放,这与该聚合物在培养中与中性粒细胞接触时释放的放射性标记物质的量相当。在类似条件下,相应的聚醚材料(TDI/PTMO/ED)未释放出大量的放射性标记。(摘要截断于250字)

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