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A microfluidic co-culture system to monitor tumor-stromal interactions on a chip

机译:一种微流体共培养系统可监控芯片上的肿瘤-基质相互作用

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摘要

The living cells are arranged in a complex natural environment wherein they interact with extracellular matrix and other neighboring cells. Cell-cell interactions, especially those between distinct phenotypes, have attracted particular interest due to the significant physiological relevance they can reveal for both fundamental and applied biomedical research. To study cell-cell interactions, it is necessary to develop co-culture systems, where different cell types can be cultured within the same confined space. Although the current advancement in lab-on-a-chip technology has allowed the creation of in vitro models to mimic the complexity of in vivo environment, it is still rather challenging to create such co-culture systems for easy control of different colonies of cells. In this paper, we have demonstrated a straightforward method for the development of an on-chip co-culture system. It involves a series of steps to selectively change the surface property for discriminative cell seeding and to induce cellular interaction in a co-culture region. Bone marrow stromal cells (HS5) and a liver tumor cell line (HuH7) have been used to demonstrate this co-culture model. The cell migration and cellular interaction have been analyzed using microscopy and biochemical assays. This co-culture system could be used as a disease model to obtain biological insight of pathological progression, as well as a tool to evaluate the efficacy of different drugs for pharmaceutical studies.
机译:活细胞被安排在复杂的自然环境中,其中它们与细胞外基质和其他邻近细胞相互作用。细胞间的相互作用,特别是不同表型之间的相互作用,由于它们可以为基础和应用生物医学研究揭示出显着的生理相关性,因此引起了人们的特别关注。为了研究细胞之间的相互作用,有必要建立共培养系统,在同一封闭空间内可以培养不同类型的细胞。尽管当前芯片实验室技术的进步已允许创建体外模型来模拟体内环境的复杂性,但是创建这样的共培养系统以轻松控制不同细胞集落仍然是相当具有挑战性的。在本文中,我们展示了一种开发片上共培养系统的简单方法。它涉及一系列步骤,以选择性地改变表面性质以区分细胞,并在共培养区诱导细胞相互作用。骨髓基质细胞(HS5)和肝肿瘤细胞系(HuH7)已用于证明此共培养模型。已经使用显微镜和生化测定法分析了细胞迁移和细胞相互作用。该共培养系统可以用作疾病模型,以获取病理进展的生物学见解,也可以用作评估不同药物在药物研究中功效的工具。

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