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导向的、多聚体的 L1 细胞黏附分子生物界面:一种增强二维和三维聚合物基底上神经元和神经干细胞功能的方法。

Oriented, multimeric biointerfaces of the L1 cell adhesion molecule: an approach to enhance neuronal and neural stem cell functions on 2-D and 3-D polymer substrates.

机构信息

Department of Biomedical Engineering, Rutgers University, 599 Taylor Road, Piscataway, NJ 08854, USA.

出版信息

Biointerphases. 2012 Dec;7(1-4):22. doi: 10.1007/s13758-012-0022-1. Epub 2012 Mar 6.

Abstract

This article focuses on elucidating the key presentation features of neurotrophic ligands at polymer interfaces. Different biointerfacial configurations of the human neural cell adhesion molecule L1 were established on two-dimensional films and three-dimensional fibrous scaffolds of synthetic tyrosine-derived polycarbonate polymers and probed for surface concentrations, microscale organization, and effects on cultured primary neurons and neural stem cells. Underlying polymer substrates were modified with varying combinations of protein A and poly-D-lysine to modulate the immobilization and presentation of the Fc fusion fragment of the extracellular domain of L1 (L1-Fc). When presented as an oriented and multimeric configuration from protein A-pretreated polymers, L1-Fc significantly increased neurite outgrowth of rodent spinal cord neurons and cerebellar neurons as early as 24 h compared to the traditional presentation via adsorption onto surfaces treated with poly-D-lysine. Cultures of human neural progenitor cells screened on the L1-Fc/polymer biointerfaces showed significantly enhanced neuronal differentiation and neuritogenesis on all protein A oriented substrates. Notably, the highest degree of βIII-tubulin expression for cells in 3-D fibrous scaffolds were observed in protein A oriented substrates with PDL pretreatment, suggesting combined effects of cell attachment to polycationic charged substrates with subcellular topography along with L1-mediated adhesion mediating neuronal differentiation. Together, these findings highlight the promise of displays of multimeric neural adhesion ligands via biointerfacially engineered substrates to "cooperatively" enhance neuronal phenotypes on polymers of relevance to tissue engineering.

摘要

本文重点阐述了神经营养因子在聚合物界面上的关键表现特征。在二维薄膜和三维纤维支架上构建了人神经细胞黏附分子 L1 的不同生物界面构型,研究了其表面浓度、微尺度组织以及对培养的原代神经元和神经干细胞的影响。聚合物基底通过不同组合的蛋白 A 和聚-D-赖氨酸进行修饰,以调节 L1 胞外域 Fc 融合片段(L1-Fc)的固定和呈现。当以蛋白 A 预处理聚合物呈现定向和多聚体构型时,L1-Fc 可显著增加 24 小时内啮齿动物脊髓神经元和小脑神经元的突起生长,而传统的通过吸附到用聚-D-赖氨酸处理的表面上的方式则不行。在 L1-Fc/聚合物生物界面上筛选的人神经祖细胞培养物显示,在所有蛋白 A 定向的基质上,神经元分化和突起形成明显增强。值得注意的是,在具有 PDL 预处理的蛋白 A 定向基质上,3-D 纤维支架中细胞的 βIII-微管蛋白表达水平最高,这表明细胞附着到带正电荷的多聚阳离子基质上的亚细胞形貌与 L1 介导的黏附共同促进神经元分化。总之,这些发现强调了通过生物界面工程化底物展示多聚体神经黏附配体的潜力,以“协同”增强与组织工程相关的聚合物上的神经元表型。

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