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生产和体外评价用于神经修复的大孔、细胞包封海藻酸盐纤维。

Production and in vitro evaluation of macroporous, cell-encapsulating alginate fibres for nerve repair.

机构信息

The University of Queensland, Pharmacy Australia Centre of Excellence, 20 Cornwall Street, Woolloongabba, Brisbane QLD 4102, Australia.

Faculty of Science, Engineering and Computing, Kingston University, Kingston upon Thames, Surrey KT1 2EE, UK.

出版信息

Mater Sci Eng C Mater Biol Appl. 2017 Apr 1;73:653-664. doi: 10.1016/j.msec.2016.12.016. Epub 2016 Dec 14.

Abstract

The prospects for successful peripheral nerve repair using fibre guides are considered to be enhanced by the use of a scaffold material, which promotes attachment and proliferation of glial cells and axonal regeneration. Macroporous alginate fibres were produced by extraction of gelatin particle porogens from wet spun fibres produced using a suspension of gelatin particles in 1.5% w/v alginate solution. Gelatin loading of the starting suspension of 40.0, 57.0, and 62.5% w/w resulted in gelatin loading of the dried alginate fibres of 16, 21, and 24% w/w respectively. Between 45 and 60% of the gelatin content of hydrated fibres was released in 1h in distilled water at 37°C, leading to rapid formation of a macroporous structure. Confocal laser scanning microscopy (CLSM) and image processing provided qualitative and quantitative analysis of mean equivalent macropore diameter (48-69μm), pore size distribution, estimates of maximum porosity (14.6%) and pore connectivity. CLSM also revealed that gelatin residues lined the macropore cavities and infiltrated into the body of the alginate scaffolds, thus, providing cell adhesion molecules, which are potentially advantageous for promoting growth of glial cells and axonal extension. Macroporous alginate fibres encapsulating nerve cells [primary rat dorsal root ganglia (DRGs)] were produced by wet spinning alginate solution containing dispersed gelatin particles and DRGs. Marked outgrowth was evident over a distance of 150μm at day 11 in cell culture, indicating that pores and channels created within the alginate hydrogel were providing a favourable environment for neurite development. These findings indicate that macroporous alginate fibres encapsulating nerve cells may provide the basis of a useful strategy for nerve repair.

摘要

利用纤维引导物成功修复周围神经的前景被认为可以通过使用支架材料来增强,该材料促进神经胶质细胞的附着和增殖以及轴突再生。通过从由在 1.5%w/v 藻酸盐溶液中的明胶颗粒悬浮液中纺出的湿纺纤维中提取明胶颗粒成孔剂来生产大孔海藻酸盐纤维。起始悬浮液中明胶的负载为 40.0、57.0 和 62.5%w/w 时,分别导致干燥的海藻酸盐纤维中的明胶负载为 16、21 和 24%w/w。在 37°C 的蒸馏水中,在 1h 内释放了水合纤维中明胶含量的 45-60%,导致大孔结构的快速形成。共焦激光扫描显微镜(CLSM)和图像处理提供了平均等效大孔直径(48-69μm)、孔径分布、最大孔隙率(14.6%)和孔连通性的定性和定量分析。CLSM 还显示明胶残留物排列在大孔腔中并渗透到海藻酸盐支架的主体中,从而提供了细胞粘附分子,这对于促进神经胶质细胞的生长和轴突延伸可能是有利的。通过在含有分散的明胶颗粒和 DRG 的藻酸盐溶液中进行湿法纺丝来生产包埋神经细胞(原代大鼠背根神经节(DRG))的大孔海藻酸盐纤维。在细胞培养中第 11 天,在 150μm 的距离上明显可见生长,表明在海藻酸盐水凝胶内创建的孔和通道为神经突的发育提供了有利的环境。这些发现表明,包埋神经细胞的大孔海藻酸盐纤维可能为神经修复提供有用策略的基础。

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