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A three-dimensional flow control concept for single-cell experiments on a microchip. 2. Fluorescein diacetate metabolism and calcium mobilization in a single yeast cell as stimulated by glucose and pH changes

机译:在微芯片上进行单细胞实验的三维流动控制概念。 2.受葡萄糖和pH变化刺激,单个酵母细胞中的双乙酸荧光素代谢和钙动员

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Using a three-dimensional flow control concept to manipulate and retain a single yeast cell in a microchip, we were able to study the kinetics of intracellular metabolism and calcium mobilization at the single-cell level, as stimulated by glucose and pH changes. As a model study, the fluorogenic substrate fluorescein diacetate (FDA) was chosen to study how the intracellular carboxylesterase metabolize it. A single yeast cell was first cultured in the microchip. Thereafter, under a constant concentration of FDA, influx of FDA into the yeast cell occurred and FDA was hydrolyzed or metabolized. It was found that changes in both pH and glucose stimulated the FDA metabolism in a yeast cell, and the stimuli can elicit multiple responses from the cell. Since it was carried out within the microchip, the whole experiment on one single yeast cell could last for as long as 10 h. The dormant cell, budding cell, and pretreated budding cell (in low-pH buffer) of yeast resulted in different responses. Experimental data provided details on the FDA metabolism at the single-cell level and revealed strong correlations between FDA metabolism and calcium mobilization. Furthermore, efflux of the FDA metabolite fluorescein could start spontaneously if there was glucose in the medium. The experiments on a single cell were of the "human cell conservation" style because the cell responded to the reagent changes implemented by the human researcher. A mathematical model was also developed to study the influx-hydrolysis-efflux processes of the FDA metabolism using single-cell fluorescent data. These long overdue single-cell experiments are now rendered possible using the three-dimensional flow control in the microchip.
机译:使用三维流动控制概念来操纵并在微芯片中保留单个酵母细胞,我们能够研究葡萄糖和pH值变化刺激的单细胞水平的细胞内代谢和钙动员的动力学。作为模型研究,选择了荧光底物二乙酸荧光素(FDA)来研究细胞内羧酸酯酶如何代谢它。首先在微芯片中培养单个酵母细胞。此后,在恒定浓度的FDA下,FDA流入酵母细胞,并且FDA水解或代谢。发现pH和葡萄糖的变化都刺激了酵母细胞中的FDA代谢,并且刺激可以引起细胞的多种反应。由于它是在微芯片内进行的,因此在单个酵母细胞上进行的整个实验可能会持续长达10小时。酵母的休眠细胞,出芽细胞和预处理的出芽细胞(在低pH缓冲液中)导致不同的响应。实验数据提供了有关单细胞水平FDA代谢的详细信息,并揭示了FDA代谢与钙动员之间的密切关系。此外,如果培养基中存在葡萄糖,FDA代谢物荧光素的流出可能会自发开始。在单个细胞上进行的实验属于“人类细胞保守”风格,因为该细胞对人类研究人员实施的试剂变化做出了反应。还开发了数学模型,以使用单细胞荧光数据研究FDA代谢的流入-水解-流出过程。现在,使用微芯片中的三维流控制,这些早就该进行的单细胞实验成为可能。

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