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补充了羟乙基纤维素的壳聚糖-甘油磷酸溶液的细胞相容性凝胶形成归因于乙二醛的存在。

Cytocompatible gel formation of chitosan-glycerol phosphate solutions supplemented with hydroxyl ethyl cellulose is due to the presence of glyoxal.

作者信息

Hoemann C D, Chenite A, Sun J, Hurtig M, Serreqi A, Lu Z, Rossomacha E, Buschmann M D

机构信息

Department of Chemical Engineering, Ecole Polytechnique, PO Box 6079, Station Centre-Ville, Montreal, Quebec, Canada H3C 3A7.

出版信息

J Biomed Mater Res A. 2007 Nov;83(2):521-9. doi: 10.1002/jbm.a.31365.

Abstract

To deliver and retain viable repair cells in a surgically prepared cartilage lesion, we previously developed an adhesive in situ-gelling cell carrier by suspending cells in a solution of hydroxyethyl cellulose (HEC), which was then mixed with chitosan-glycerol phosphate to form a chitosan-GP/HEC gel. The purpose of this study was to elucidate the mechanism of gelation to maximally control gel time and viability of encapsulated cells. We analyzed the role of osmolality, pH, gelation temperature, gel shrinkage, and HEC. A chitosan-GP solution at pH 6.8 with cytocompatible osmotic pressure (419 mOsm/kg) was achieved by lowering disodium GP concentration from 370 to 135 mM. This solution was still thermogelling but only at 73 degrees C. We next discovered that glyoxal, a common additive in ether cellulose manufacturing, was responsible for chitosan gelation. Monolayer cells survived and proliferated in up to 1 mM of glyoxal, however only a very narrow range of glyoxal concentration in chitosan-GP/HEC, 0.1-0.15 mM, permitted gel formation, cell survival, and cell proliferation. Chitosan gels containing HEC required slightly less glyoxal to solidify. Chitosan-GP/HEC loaded with viable chondrocytes formed an adhesive seal with ex vivo mosaic arthroplasty defects from sheep knee joints. In mosaic arthroplasty defects of live sheep, bleeding occurred beneath part of the hydrogel carrier, and the gel was cleared after 1 month in vivo. These data indicate that chitosan-GP/HEC is suitable as an adhesive and injectable delivery vehicle for clinical orthopedic applications involving single use treatments that guide acute cartilage repair processes.

摘要

为了在手术制备的软骨损伤部位递送并保留有活力的修复细胞,我们之前开发了一种原位凝胶化的黏附性细胞载体,方法是将细胞悬浮于羟乙基纤维素(HEC)溶液中,然后与壳聚糖 - 甘油磷酸混合形成壳聚糖 - GP/HEC凝胶。本研究的目的是阐明凝胶化机制,以最大程度地控制凝胶时间和包封细胞的活力。我们分析了渗透压、pH值、凝胶化温度、凝胶收缩和HEC的作用。通过将甘油磷酸二钠浓度从370 mM降至135 mM,获得了pH值为6.8且具有细胞相容性渗透压(419 mOsm/kg)的壳聚糖 - GP溶液。该溶液仍具有热凝胶化特性,但仅在73℃时发生。接下来我们发现,乙二醛这种醚纤维素制造中的常见添加剂是壳聚糖凝胶化的原因。单层细胞在高达1 mM的乙二醛中能够存活并增殖,然而在壳聚糖 - GP/HEC中,只有非常窄的乙二醛浓度范围(0.1 - 0.15 mM)允许凝胶形成、细胞存活和细胞增殖。含有HEC的壳聚糖凝胶固化所需的乙二醛略少。负载有活力软骨细胞的壳聚糖 - GP/HEC与绵羊膝关节的离体镶嵌式关节成形术缺损形成了黏附性密封。在活羊的镶嵌式关节成形术缺损中,水凝胶载体部分下方出现出血,且凝胶在体内1个月后被清除。这些数据表明,壳聚糖 - GP/HEC适合作为一种黏附性和可注射的递送载体,用于涉及单次使用治疗以指导急性软骨修复过程的临床骨科应用。

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