Carlson Grady E, Martin Eric W, Burdick Monica M
Department of Chemical and Biomolecular Engineering, Russ College of Engineering and Technology, Ohio University.
J Vis Exp. 2013 Sep 4(79):50604. doi: 10.3791/50604.
Multi-color immunofluorescence microscopy to detect specific molecules in the cell membrane can be coupled with parallel plate flow chamber assays to investigate mechanisms governing cell adhesion under dynamic flow conditions. For instance, cancer cells labeled with multiple fluorophores can be perfused over a potentially reactive substrate to model mechanisms of cancer metastasis. However, multi-channel single camera systems and color cameras exhibit shortcomings in image acquisition for real-time live cell analysis. To overcome these limitations, we used a dual camera emission splitting system to simultaneously capture real-time image sequences of fluorescently labeled cells in the flow chamber. Dual camera emission splitting systems filter defined wavelength ranges into two monochrome CCD cameras, thereby simultaneously capturing two spatially identical but fluorophore-specific images. Subsequently, psuedocolored one-channel images are combined into a single real-time merged sequence that can reveal multiple target molecules on cells moving rapidly across a region of interest.
用于检测细胞膜中特定分子的多色免疫荧光显微镜可与平行板流动腔分析相结合,以研究动态流动条件下细胞黏附的机制。例如,用多种荧光团标记的癌细胞可以灌注到潜在的反应性底物上,以模拟癌症转移的机制。然而,多通道单相机系统和彩色相机在实时活细胞分析的图像采集方面存在缺点。为了克服这些限制,我们使用了双相机发射分光系统来同时捕获流动腔中荧光标记细胞的实时图像序列。双相机发射分光系统将定义的波长范围过滤到两个单色CCD相机中,从而同时捕获两个空间相同但荧光团特异性的图像。随后,伪彩色单通道图像被组合成一个单一的实时合并序列,该序列可以揭示在感兴趣区域快速移动的细胞上的多个靶分子。