Biomicrofluidics. 2010 Dec 30;4(4):43009. doi: 10.1063/1.3491470.
A method for monitoring the biological exocytotic phenomena on a microfluidic system was proposed. A microfluidic device coupled with functionalities of fluorescence imaging and amperometric detection has been developed to enable the real-time monitoring of the exocytotic events. Exocytotic release of single SH-SY5Y neuroblastoma cells was studied. By staining the cells located on integrated microelectrodes with naphthalene-2,3-dicarboxaldehyde, punctuate fluorescence consistent with localization of neurotransmitters stored in vesicles was obtained. The stimulated exocytotic release was successfully observed at the surface of SH-SY5Y cells without refitting the commercial inverted fluorescence microscope. Spatially and temporally resolved exocytotic events from single cells on a microfluidic device were visualized in real time using fluorescence microscopy and were amperometrically recorded by the electrochemical system simultaneously. This coupled technique is simple and is hoped to provide new insights into the mechanisms responsible for the kinetics of exocytosis.
提出了一种在微流控系统上监测生物胞吐现象的方法。开发了一种微流控装置,结合荧光成像和安培检测功能,实现了对胞吐事件的实时监测。研究了单个 SH-SY5Y 神经母细胞瘤细胞的胞吐释放。通过用萘-2,3-二醛对位于集成微电极上的细胞进行染色,获得了与囊泡中储存的神经递质定位一致的点状荧光。在不重新装配商用倒置荧光显微镜的情况下,成功地观察到 SH-SY5Y 细胞表面的刺激胞吐释放。使用荧光显微镜实时可视化微流控装置上单个细胞的时空分辨胞吐事件,并通过电化学系统同时进行安培记录。这种耦合技术简单,有望为胞吐动力学的机制提供新的见解。