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Micropatterned co-culture of hepatocyte spheroids layered on non-parenchymal cells to understand heterotypic cellular interactions

机译:在非实质细胞上分层的肝细胞球体的微模式共培养以了解异型细胞相互作用

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摘要

Microfabrication and micropatterning techniques in tissue engineering offer great potential for creating and controlling cellular microenvironments including cell–matrix interactions, soluble stimuli and cell–cell interactions. Here, we present a novel approach to generate layered patterning of hepatocyte spheroids on micropatterned non-parenchymal feeder cells using microfabricated poly(ethylene glycol) (PEG) hydrogels. Micropatterned PEG-hydrogel-treated substrates with two-dimensional arrays of gelatin circular domains (ϕ = 100 μm) were prepared by photolithographic method. Only on the critical structure of PEG hydrogel with perfect protein rejection, hepatocytes were co-cultured with non-parenchymal cells to be led to enhanced hepatocyte functions. Then, we investigated the mechanism of the functional enhancement in co-culture with respect to the contributions of soluble factors and direct cell–cell interactions. In particular, to elucidate the influence of soluble factors on hepatocyte function, hepatocyte spheroids underlaid with fibroblasts (NIH/3T3 mouse fibroblasts) or endothelial cells (BAECs: bovine aortic endothelial cells) were compared with physically separated co-culture of hepatocyte monospheroids with NIH3T3 or BAEC using trans-well culture systems. Our results suggested that direct heterotypic cell-to-cell contact and soluble factors, both of these between hepatocytes and fibroblasts, significantly enhanced hepatocyte functions. In contrast, direct heterotypic cell-to-cell contact between hepatocytes and endothelial cells only contributed to enhance hepatocyte functions. This patterning technique can be a useful experimental tool for applications in basic science, drug screening and tissue engineering, as well as in the design of artificial liver devices.
机译:组织工程学中的微细加工和微图案技术为创造和控制细胞微环境提供了巨大的潜力,包括细胞-基质相互作用,可溶性刺激物和细胞-细胞相互作用。在这里,我们提出了一种使用微细加工的聚乙二醇(PEG)水凝胶在微图案化的非实质饲养细胞上生成肝细胞球体的分层图案的新方法。通过光刻法制备具有明胶环状结构域二维阵列(φ= 100μm)的微图案化PEG-水凝胶处理的基质。仅在具有完美蛋白质排斥的PEG水凝胶的关键结构上,肝细胞才与非实质细胞共培养,从而导致增强的肝细胞功能。然后,我们针对可溶性因子和直接细胞间相互作用的作用,研究了共培养功能增强的机制。特别是,为了阐明可溶性因子对肝细胞功能的影响,将成纤维细胞(NIH / 3T3小鼠成纤维细胞)或内皮细胞(BAEC:牛主动脉内皮细胞)和肝细胞单球体与NIH3T3物理分离共培养的肝细胞球体进行了比较。或使用跨孔培养系统的BAEC。我们的研究结果表明,肝细胞和成纤维细胞之间直接的异型细胞间接触和可溶性因子都显着增强了肝细胞的功能。相反,肝细胞与内皮细胞之间的异型细胞直接接触仅有助于增强肝细胞功能。这种图案化技术可以用作基础科学,药物筛选和组织工程以及人造肝脏设备设计中的有用实验工具。

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