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首页> 外文期刊>BMC Systems Biology >Towards embedding Caco-2 model of gut interface in a microfluidic device to enable multi-organ models for systems biology
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Towards embedding Caco-2 model of gut interface in a microfluidic device to enable multi-organ models for systems biology

机译:将内脏接口的Caco-2模型嵌入微流控设备中,以实现用于系统生物学的多器官模型

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A cancer cell line originating from human epithelial colorectal adenocarcinoma (Caco-2 cells) serves as a high capacity model for a preclinical screening of drugs. Recent need for incorporating barrier tissue into multi-organ chips calls for inclusion of Caco-2 cells into microperfused environment. This article describes a series of systems biology insights obtained from comparing Caco-2 models cells grown as conventional 2D layer and in a microfluidic chip. When basic electrical parameters of Caco-2 monolayers were evaluated using impedance spectrometry and MTT assays, no differences were noted. On the other hand, the microarray profiling of mRNAs and miRNAs revealed that grows on a microfluidic chip leads to the change in the production of specific miRNA, which regulate a set of genes for cell adhesion molecules (CAMs), and provide for more complete differentiation of Caco-2 monolayer. Moreover, the sets of miRNAs secreted at the apical surface of Caco-2 monolayers grown in conventional 2D culture and in microfluidic device differ. When integrated into a multi-tissue platform, Caco-2 cells may aid in generating insights into complex pathophysiological processes, not possible to dissect in conventional cultures.
机译:源自人上皮结肠直肠腺癌(Caco-2细胞)的癌细胞系可作为药物临床前筛选的高容量模型。最近需要将屏障组织整合到多器官芯片中,这要求将Caco-2细胞包含在微灌流环境中。本文介绍了通过比较以常规2D层和微流控芯片形式生长的Caco-2模型细胞而获得的一系列系统生物学见解。当使用阻抗谱和MTT分析法评估Caco-2单层的基本电参数时,没有发现差异。另一方面,mRNA和miRNA的微阵列分析显示,在微流体芯片上生长会导致特定miRNA产生量的变化,从而调节细胞粘附分子(CAMs)的一组基因,并提供更完全的分化Caco-2单层。此外,在常规2D培养和微流控设备中生长的Caco-2单层顶表面分泌的miRNA的集合也不同。当整合到多组织平台中时,Caco-2细胞可能有助于产生对复杂病理生理过程的了解,而这在常规培养中是不可能分解的。

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