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A closer look at neuron interaction with track-etched microporous membranes

机译:仔细研究神经元与刻蚀微孔膜的相互作用

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摘要

Microporous membranes support the growth of neurites into and through micro-channels, providing a different type of neural growth platform to conventional dish cultures. Microporous membranes are used to support various types of culture, however, the role of pore diameter in relation to neurite growth through the membrane has not been well characterised. In this study, the human cell line (SH-SY5Y) was differentiated into neuron-like cells and cultured on track-etched microporous membranes with pore and channel diameters selected to accommodate neurite width (0.8 µm to 5 µm). Whilst neurites extended through all pore diameters, the extent of neurite coverage on the non-seeded side of the membranes after 5 days in culture was found to be directly proportional to channel diameter. Neurite growth through membrane pores reduced significantly when neural cultures were non-confluent. Scanning electron microscopy revealed that neurites bridged pores and circumnavigated pore edges – such that the overall likelihood of a neurite entering a pore channel was decreased. These findings highlight the role of pore diameter, cell sheet confluence and contact guidance in directing neurite growth through pores and may be useful in applications that seek to use physical substrates to maintain separate neural populations whilst permitting neurite contact between cultures.
机译:微孔膜支持神经突进入微通道并通过微通道生长,从而为常规培养皿培养提供了不同类型的神经生长平台。微孔膜用于支持各种类型的培养,但是,孔径与通过膜的神经突生长相关的作用尚未得到很好的表征。在这项研究中,人类细胞系(SH-SY5Y)分化为神经元样细胞,并在径迹蚀刻的微孔膜上进行培养,其孔和通道直径选择为适应神经突宽度(0.8μm至5μm)。虽然神经突延伸通过所有孔径,但是在培养5天后发现神经突在膜的非种子侧的覆盖程度与通道直径成正比。当神经培养物不融合时,通过膜孔的神经突生长显着减少。扫描电子显微镜显示,神经突桥接孔并绕过孔边缘-这样就降低了神经突进入孔道的总体可能性。这些发现突出了孔径,细胞片汇合和接触引导在引导神经突通过孔生长中的作用,并且在寻求使用物理底物维持单独的神经种群同时允许培养物之间的神经突接触的应用中可能有用。

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