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人诱导多能干细胞中糖酵解和线粒体呼吸的芯片分析

On-chip analysis of glycolysis and mitochondrial respiration in human induced pluripotent stem cells.

作者信息

Fuchs Stefanie, van Helden Ruben W J, Wiendels Maury, de Graaf Mees N S, Orlova Valeria V, Mummery Christine L, van Meer Berend J, Mayr Torsten

机构信息

Institute of Analytical Chemistry and Food Chemistry, Graz University of Technology, Graz, Austria.

Department of Anatomy & Embryology, Leiden University Medical Center, Leiden, Netherlands.

出版信息

Mater Today Bio. 2022 Oct 31;17:100475. doi: 10.1016/j.mtbio.2022.100475. eCollection 2022 Dec 15.

Abstract

Recent advances in microfluidic engineering allow the creation of microenvironments in which human cells can be cultured under (patho-)physiological conditions with greater reality than standard plastic tissue culture plates. Microfluidic devices, also called Organs-on-Chip (OoC), allow complex engineering of the cellular compartment, yielding designs in which microfluidic flow can be precisely controlled. However, it is important that cellular physiology is not only controlled but can also be monitored in these devices. Here, we integrated oxygen and pH sensors into microfluidics, allowing close monitoring of the extracellular flux from the cells, enabling constant assessment of features such as glycolysis and mitochondrial oxidative phosphorylation . Using human-induced pluripotent stem cells (hiPSCs) as an exemplar of a highly metabolic and relatively challenging cell type to maintain, we showed that monitoring the extracellular environment allowed rapid optimization of the seeding protocol. Based on the measurements, we implemented earlier and more frequent media refreshment to counteract the rapid acidification and depletion of oxygen. The integrated sensors showed that hiPSCs in the devices exhibited mitochondrial and glycolytic capacity similar to that measured with the Seahorse extracellular flux system, the most widely used standard for these types of assays in conventional cell culture. Under both conditions, hiPSCs showed greater reliance on glycolysis than mitochondrial OXPHOS and the absolute values obtained were similar. These results thus pave the way for the assessment of cell metabolism under conditions of fluidic flow with the same precision and relevance as current standard static cell cultures.

摘要

微流控工程的最新进展使得能够创建微环境,在其中人类细胞可以在(病理)生理条件下培养,比标准塑料组织培养板更接近真实情况。微流控设备,也称为芯片上的器官(OoC),允许对细胞区室进行复杂的工程设计,产生能够精确控制微流的设计。然而,重要的是,在这些设备中,细胞生理学不仅要得到控制,而且还要能够被监测。在这里,我们将氧气和pH传感器集成到微流控系统中,从而能够密切监测细胞的细胞外通量,持续评估糖酵解和线粒体氧化磷酸化等特征。我们以人类诱导多能干细胞(hiPSC)作为一种高代谢且相对难以维持的细胞类型的范例,表明监测细胞外环境能够快速优化接种方案。基于这些测量结果,我们实施了更早且更频繁的培养基更新,以抵消快速的酸化和氧气消耗。集成传感器显示,设备中的hiPSC表现出的线粒体和糖酵解能力与使用海马细胞外通量系统测量的结果相似,海马细胞外通量系统是传统细胞培养中这类检测最广泛使用的标准。在这两种条件下,hiPSC对糖酵解的依赖都大于线粒体氧化磷酸化,并且获得的绝对值相似。因此,这些结果为在流体流动条件下以与当前标准静态细胞培养相同的精度和相关性评估细胞代谢铺平了道路。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/f9ab/9647220/31e6ffb5b51f/ga1.jpg

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