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A microfluidic approach for experimentally modelling the intercellular coupling system of a mammalian circadian clock at single-cell level

机译:一种微流体方法,用于在单细胞水平下进行实验模拟哺乳动物昼夜昼夜时钟的细胞间耦合系统

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In mammals, it is believed that the intercellular coupling mechanism between neurons in the suprachiasmatic nucleus (SCN) confers robustness and distinguishes the central clock from peripheral circadian oscillators. Current in vitro culturing methods used in Petri dishes to study intercellular coupling by exogenous factors invariably cause perturbations, such as simple media changes. Here, we design a microfluidic device to quantitatively study the intercellular coupling mechanism of circadian clock at the single cell level, and demonstrate that vasoactive intestinal peptide (VIP) induced coupling in clock mutant Cry1-/- mouse adult fibroblasts engineered to express the VIP receptor, VPAC2, is sufficient to synchronize and maintain robust circadian oscillations. Our study provides a proof-of-concept platform to reconstitute the intercellular coupling system of the central clock using uncoupled, single fibroblast cells in vitro, to mimic SCN slice cultures ex vivo and mouse behavior in vivo phenotypically. Such a versatile microfluidic platform may greatly facilitate the studies of intercellular regulation networks, and provide new insights into the coupling mechanisms of the circadian clock.
机译:在哺乳动物中,据信神经元之间的细胞间偶联机制在高温核(SCN)中的细胞间偶联机制(SCN)赋予鲁棒性,并将中心钟与外围昼夜周边振荡器区分开来。电流在培养皿中使用的体外培养方法,以通过外源因素研究细胞间偶联因子扰动,例如简单的介质变化。在这里,我们设计了一种微流体装置,以定量地研究昼夜节拍时钟的细胞间耦合机制在单个细胞水平上,并证明血管活性肠肽(VIP)诱导在时钟突变体Cry1 - / - 小鼠成年成纤维细胞中的耦合,以表达振作受体。 VPAC2足以同步和维护强大的昼夜振荡。我们的研究提供了一种概念概念平台,用于将中心时钟的间细胞间耦合系统重新替换,在体外使用未替换的单成纤维细胞,以模拟SCN切片培养物以体内的体内和小鼠行为。这种多功能的微流体平台可以极大地促进细胞间调节网络的研究,并为昼夜钟表的耦合机制提供新的见解。

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