The Garvan Institute of Medical Research, 384 Victoria Street, Sydney, New South Wales 2010, Australia.
Traffic. 2010 Apr;11(4):429-39. doi: 10.1111/j.1600-0854.2010.01039.x. Epub 2010 Jan 12.
The regulated trafficking or exocytosis of cargo-containing vesicles to the cell surface is fundamental to all cells. By coupling the technology of fluorescently tagged fusion proteins with total internal reflection fluorescence microscopy (TIRFM), it is possible to achieve the high spatio-temporal resolution required to study the dynamics of sub-plasma membrane vesicle trafficking and exocytosis. TIRFM has been used in a number of cell types to visualize and dissect the various steps of exocytosis revealing how molecules identified via genetic and/or biochemical approaches are involved in the regulation of this process. Here, we summarize the contribution of TIRFM to our understanding of the mechanism of exocytosis and discuss the novel methods of analysis that are required to exploit the large volumes of data that can be produced using this technique.
货物包含囊泡的调节运输或胞吐作用到细胞膜表面对于所有细胞都是基本的。通过将荧光标记融合蛋白的技术与全内反射荧光显微镜(TIRFM)相结合,可以实现研究亚质膜囊泡运输和胞吐作用动力学所需的高时空分辨率。TIRFM 已被用于多种细胞类型来可视化和剖析胞吐作用的各个步骤,揭示了通过遗传和/或生化方法鉴定的分子如何参与该过程的调节。在这里,我们总结了 TIRFM 对我们理解胞吐作用机制的贡献,并讨论了利用该技术产生的大量数据所需的新的分析方法。
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