首页> 美国卫生研究院文献>Tissue Engineering. Part C Methods >Engineering an Integrated Cellular Interface in Three-Dimensional Hydrogel Cultures Permits Monitoring of Reciprocal Astrocyte and Neuronal Responses
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Engineering an Integrated Cellular Interface in Three-Dimensional Hydrogel Cultures Permits Monitoring of Reciprocal Astrocyte and Neuronal Responses

机译:在三维水凝胶培养中设计集成的细胞界面可监测相互的星形胶质细胞和神经元反应

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摘要

This study reports a new type of three-dimensional (3D) tissue model for studying interactions between cell types in collagen hydrogels. The aim was to create a 3D cell culture model containing separate cell populations in close proximity without the presence of a mechanical barrier, and demonstrate its relevance to modeling the axon growth-inhibitory cellular interfaces that develop in the central nervous system (CNS) in response to damage. This provides a powerful new tool to determine which aspects of the astroglial scar response and subsequent neuronal regeneration inhibition are determined by the presence of the other cell types. Astrocytes (CNS glia) and dissociated dorsal root ganglia (DRG; containing neurons and peripheral nervous system [PNS] glia) were seeded within collagen solution at 4°C in adjacent chambers of a stainless steel mould, using cells cultured from wild-type or green fluorescent protein expressing rats, to track specific populations. The divider between the chambers was removed using a protocol that allowed the gels to integrate without mixing of the cell populations. Following setting of the gels, they were maintained in culture for up to 15 days. Reciprocal astrocyte and neuronal responses were monitored using confocal microscopy and 3D image analysis. At DRG:astrocyte interfaces, by 5 days there was an increase in the number of astrocytes at the interface followed by hypertrophy and increased glial fibrillary acidic protein expression at 10 and 15 days, indicative of reactive gliosis. Neurons avoided crossing DRG:astrocyte interfaces, and neuronal growth was restricted to the DRG part of the gel. By contrast, neurons were able to grow freely across DRG:DRG interfaces, demonstrating the absence of a mechanical barrier. These results show that in a precisely controlled 3D environment, an interface between DRG and astrocyte cultures is sufficient to trigger reactive gliosis and inhibition of neuronal regeneration across the interface. Different aspects of the astrocyte response could be independently monitored, providing an insight into the formation of a glial scar. This technology has wide potential for researchers wishing to maintain and monitor interactions between adjacent cell populations in 3D culture.
机译:这项研究报告了一种新型的三维(3D)组织模型,用于研究胶原蛋白水凝胶中细胞类型之间的相互作用。目的是创建一个3D细胞培养模型,该模型包含紧密相邻且没有机械屏障的单独细胞群,并证明其与建模响应中枢神经系统(CNS)中发育的轴突生长抑制性细胞界面的相关性损坏。这提供了一个强大的新工具,可以确定星形胶质瘢痕反应和随后的神经元再生抑制的哪些方面是由其他细胞类型的存在来确定的。将星形胶质细胞(CNS胶质细胞)和离体的背根神经节(DRG;包含神经元和周围神经系统[PNS]胶质细胞)接种在不锈钢模具相邻腔室中的胶原溶液中,温度为4°C,使用从野生型或绿色荧光蛋白表达大鼠,追踪特定种群。使用允许凝胶整合而不混合细胞群体的方案去除室之间的分隔物。凝胶凝结后,将其在培养物中最多保留15天。使用共聚焦显微镜和3D图像分析监测相互的星形胶质细胞和神经元反应。在DRG:星形胶质细胞界面处,到第5天时,在界面处的星形胶质细胞数量增加,随后在10天和15天出现肥大和胶质纤维酸性蛋白表达增加,表明反应性神经胶质增生。神经元避免穿越DRG:星形胶质细胞界面,并且神经元的生长仅限于凝胶的DRG部分。相比之下,神经元能够在DRG:DRG界面上自由生长,表明没有机械障碍。这些结果表明,在精确控制的3D环境中,DRG和星形胶质细胞培养物之间的界面足以触发反应性神经胶质细胞增生和跨该界面抑制神经元再生。星形胶质细胞反应的不同方面可以独立监测,从而提供了对神经胶质瘢痕形成的认识。对于希望在3D培养中维持和监视相邻细胞群体之间相互作用的研究人员来说,这项技术具有广阔的潜力。

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