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聚醚和聚酯型聚氨酯在氧化酶和水解酶作用下的生物降解性评估

Biodegradation evaluation of polyether and polyester-urethanes with oxidative and hydrolytic enzymes.

作者信息

Santerre J P, Labow R S, Duguay D G, Erfle D, Adams G A

机构信息

Department of Biomaterials, Faculty of Dentistry, University of Toronto, Ontario, Canada.

出版信息

J Biomed Mater Res. 1994 Oct;28(10):1187-99. doi: 10.1002/jbm.820281009.

Abstract

Enzyme-induced liberation of components from seven different radiolabeled polyurethanes was monitored by radiolabel counting of the incubation solutions and product isolation by high performance liquid chromatography (HPLC). The polyurethanes were selected to reflect variations in the hard-segment chemistry, soft-segment chemistry, and polyurethane hydrophilicity resulting from combinations of hydrophobic/hydrophilic soft segments. All materials were characterized using electron spectroscopy for chemical analysis, differential scanning calorimetry, size exclusion chromatography, and Fourier transform infrared spectroscopy. The material surfaces were examined both before and after incubation with enzyme and control solutions using scanning electron microscopy. Biodegradation assays were carried out at 37 degrees C using cholesterol esterase (CE) and horseradish peroxidase (HRP) under optimal pH conditions for each enzyme. The hydrolytic enzyme (CE) was effective in releasing degradation products that contained hard-segment components from some of the polyurethanes. HPLC analysis of products for a polyesterurethane synthesized with toluene diisocyanate (TDI) suggested that the bulk of the incorporated radiolabeled TDI was still covalently bonded within the cleaved chain segments of the original polymer and was not released as pure toluene diamine (TDA). The data suggest that urethane linkages in the soft-segment domains of phase separated polyetherurea-urethanes may be more prone to cleavage by CE than are the urea/urethane groups in the hard-segment domains. This could be related to the nature of the hard-segment domain structures. The oxidative enzyme (HRP) was not able to induce liberation of radiolabeled segments from either the polyether or polyester-based polyurethanes.

摘要

通过对孵育溶液进行放射性标记计数以及采用高效液相色谱法(HPLC)进行产物分离,监测了七种不同放射性标记聚氨酯中酶诱导的成分释放情况。选择这些聚氨酯是为了反映由于疏水/亲水软段组合导致的硬段化学、软段化学以及聚氨酯亲水性的变化。使用化学分析电子能谱、差示扫描量热法、尺寸排阻色谱法和傅里叶变换红外光谱法对所有材料进行了表征。在酶和对照溶液孵育前后,使用扫描电子显微镜对材料表面进行了检查。在37℃下,在每种酶的最佳pH条件下,使用胆固醇酯酶(CE)和辣根过氧化物酶(HRP)进行了生物降解试验。水解酶(CE)有效地从一些聚氨酯中释放出了含有硬段成分的降解产物。对用甲苯二异氰酸酯(TDI)合成的聚酯聚氨酯产物进行的HPLC分析表明,大部分掺入的放射性标记TDI仍共价键合在原始聚合物的裂解链段内,并未以纯甲苯二胺(TDA)的形式释放出来。数据表明,相分离聚醚脲 - 聚氨酯软段域中的脲键可能比硬段域中的脲/脲键更容易被CE裂解。这可能与硬段域结构的性质有关。氧化酶(HRP)无法诱导从聚醚或聚酯基聚氨酯中释放出放射性标记链段。

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