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首页> 外文期刊>Frontiers in Bioengineering and Biotechnology >A Theoretical and Experimental Study to Optimize Cell Differentiation in a Novel Intestinal Chip
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A Theoretical and Experimental Study to Optimize Cell Differentiation in a Novel Intestinal Chip

机译:一种优化新型肠芯片细胞分化的理论与实验研究

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Microphysiological systems have potential as test systems in studying the intestinal barrier, in which shear stress is critical for the differentiation of Caco-2 cells into enterocytes. The most commonly used in vitro gut model for intestinal barrier studies is based on trans-well cultures. Albeit useful, these culture systems lack physiological shear stress which is believed to be critical for the differentiation of Caco-2 cells into enterocytes and to form tight monolayers. Conversely, organ-on-chip models have presented themselves as a promising alternative since they provide cells with the required shear stress. To this end, a novel biocompatible 3D-printed microfluidic device was developed. In this device, Caco-2 cells were seeded under physiologically-relevant unidirectional shear stress and compared to cells cultured under gravity-driven flow. Using numerical studies, the flow rate that corresponds to the required shear stress was calculated. Experimental tests were conducted to verify the effect of this on cell differentiation. The experiments clearly showed an enhancement of cell differentiation potential in a unidirectional physiologically relevant pump-driven flow system (PDFS) as opposed to the simpler bidirectional gravity-driven flow system (GDFS). Additionally, computational modeling of an adapted design confirmed its ability to supply all cells with a more homogeneous shear stress, potentially further enhancing their differentiation. The shear stress in the adapted design can be well approximated with analytic methods, thus allowing for efficient predictions for all parameter values in the system. The developed novel microfluidic device led to the formation of a tighter monolayer and enhanced functional properties of the differentiated Caco-2 cells, which presents a promising tool for preclinical in vitro testing of drugs in an animal-free platform.
机译:微生物系统具有在研究肠道屏障时具有测试系统的潜力,其中剪切应力对于将Caco-2细胞分化成肠细胞至关重要。最常用的肠道阻隔研究中的体外肠道模型基于杂交井培养物。尽管有用的是,这些培养系统缺乏生理剪切应力,其被认为对CaCO-2细胞分化为肠细胞并形成紧密单层。相反,片上模型本身就像他们提供了具有所需剪切应力的细胞一样。为此,开发了一种新型生物相容性的3D印刷微流体装置。在该装置中,在生理相关的单向剪切应力下接种Caco-2细胞,并与在重力驱动流动下培养的细胞进行比较。使用数值研究,计算对应于所需剪切应力的流速。进行实验试验以验证该方法对细胞分化的影响。实验清楚地表明,与更简单的双向重力驱动流动系统(GDF)相比,在单向生理相关的泵驱动流系统(PDF)中的细胞分化电位的增强。另外,适应性设计的计算建模证实了能够提供更均匀的剪切应力的所有细胞,可能进一步增强它们的分化。适应设计中的剪切应力可以通过分析方法近似地近似,从而允许对系统中的所有参数值进行有效预测。开发的新型微流体装置导致形成更严格的单层和增强的分化的Caco-2细胞的功能性,这提出了一种有前途的工具,用于无动物平台中药物的临床前体外测试。

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