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山东大学学报(理学版) ›› 2016, Vol. 51 ›› Issue (1): 36-42.doi: 10.6040/j.issn.1671-9352.0.2015.219

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三维鱼类胶原支架的制备及其生物相容性研究

袁晓龙,徐彬,樊廷俊*   

  1. 中国海洋大学海洋生命学院角膜组织工程重点实验室, 山东 青岛 266003
  • 收稿日期:2015-05-12 出版日期:2016-01-16 发布日期:2016-11-29
  • 通讯作者: 樊廷俊(1964— ),男,博士,教授,博士生导师,研究方向为细胞工程与角膜组织工程. E-mail:tjfan@ouc.edu.cn E-mail:rayrock@126.com
  • 作者简介:袁晓龙(1988— ),男,博士,研究方向为角膜组织工程. E-mail:rayrock@126.com
  • 基金资助:
    国家高技术研究发展计划(863计划)资助项目(2006AA02A132)

Fabrication of a three-dimensional fish collagen scaffold and its biocompatibility characterization

YUAN Xiao-long, XU Bin, FAN Ting-jun*   

  1. Key Laboratory for Corneal Tissuse Engineering, College of Marine Life Sciences, Ocean University of China, Qingdao 266003, Shandong, China
  • Received:2015-05-12 Online:2016-01-16 Published:2016-11-29

摘要: 为了评价深海鱼类胶原蛋白用于制备组织工程角膜载体支架的可行性,首次利用鱼皮胶原蛋白进行了三维胶原支架的制备及其生物相容性研究。用源于太平洋鳕鱼(Gadus macrocephalus)的纯化鱼皮胶原蛋白,经冷冻干燥后选用1-乙基-3-(3-二甲基氨基丙基)碳二亚胺(EDC)/N-羟基丁二酰亚胺(NHS)交联剂制备出三维胶原支架,利用外观照相、光度计透光率、冰冻切片苏木紫-伊红(HE)染色及扫描电镜检测了其透明度和组织结构;在接种DiI(1,1'-dioctadecyl-3,3,3',3'-tetramethylindocarbocyanine perchlorate)荧光标记的非转染人角膜基质(HCS)细胞后,利用冰冻切片HE染色和荧光观察鉴定了细胞的迁入及在支架内的分布情况,生物相容性评价采用MTT(噻唑蓝)和免疫细胞荧光技术检测了支架对HCS细胞活力和标志蛋白及功能蛋白表达的影响。结果显示,所制备的三维胶原支架透明度极高,呈现出均匀的网格状结构,孔径大小为50~130 μm;接种HCS细胞并体外培养3 d后,发现有大量细胞迁入支架内且分布较为均匀;支架抽提物对HCS细胞活力没有任何不良影响;且迁入支架内的细胞仍保持有其标志蛋白—波形蛋白,细胞连接形成蛋白—整联蛋白β1、E-钙黏蛋白和间隙连接蛋白-43,膜运输蛋白—钠钾泵,以及抗UV蛋白—乙醛脱氢酶的阳性表达。综上所述,利用太平洋鳕鱼皮胶原蛋白制备的三维胶原支架具有良好的透明度与组织结构,不仅适合HCS细胞的顺利迁入,而且对HCS细胞具有良好的生物相容性,有望作为载体支架用于组织工程角膜的体外构建研究。

关键词: 鱼皮胶原蛋白, 人基质角膜细胞, 太平洋鳕鱼, 生物相容性, 三维胶原支架

Abstract: To verify the feasibility of deep-sea fish collagen to be utilized in fabrication of the scaffold for tissue-engineered cornea, a novel three-dimensional(3D)collagen scaffold was produced using fish skin collagen for the first time and its biocompatibility was evaluated in this study. After freeze dried fish skin collagen, purified from the skin of Gadus microcephalus, was cross-linked using N-(3-Dimethylaminopropyl)-N' -ethylcarbodiimide hydrochloride crystalline(EDC)/N-Hydroxysuccinimide(NHS), a 3D-collagen scaffold was obtained. Its transparency and histological structure were detected and identified by macroscopy, photospectrometry, hematoxylin-eosin(HE)staining of frozen sections, scanning electron microscope. After DiI(1,1'-dioctadecyl-3,3,3',3'-tetramethylindocarbocyanine perchlorate)-labeled human corneal stromal(HCS)cells were inoculated onto the scaffold, the immigration and distribution of the cells were identified by HE staining of frozen sections and fluorescent microscopy. The biocompatibility of the scaffold to HCS cells was characterized by MTT assay and immunocytofluorescent microscopy to examine the cell viability and expression patterns of marker protein and functional proteins. Our results showed that the fabricated 3D-collagen scaffold had an excellent transparency, uniform organized reticular structure with pore size of 50-130 μm. After HCS cells were 山 东 大 学 学 报 (理 学 版)第51卷 - 第1期袁晓龙,等:三维鱼类胶原支架的制备及其生物相容性研究 \=-inoculated onto the scaffold, a lot of the cells could migrate into the scaffold, and the inoculated HCS cells distributed regularly in the scaffold 3 days after cultured in vitro. Moreover, the extracts of the scaffold had no obvious adverse effects on the viability of HCS cells. The inoculated HCS cells still maintained the positive expression of the marker protein of vimentin, cell junction proteins of integrin β1, E-cadherin and connexin-43, membrane transport protein of Na+-K+-ATPase, and anti-UV protein of acetaldehyde dehydrogenase. In conclusion, the 3D-collagen scaffold fabricated from G.macrocephalus skin collagen, in good transparency and histological structure, was suitable for HCS cell immigration, and has good biocompatibility to these cells. The 3D-collagen scaffold has promising potentials to be used in the in vitro construction of tissue-engineered cornea.

Key words: human corneal stromal cell, biocompatibility, fish skin collagen, Gadus macrocephalus, 3D collagen scaffold

中图分类号: 

  • Q813
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