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用于可视化活的盘基网柄菌细胞中单个分子的成像室的制备。

Preparation of an imaging chamber for visualizing single molecules in living Dictyostelium cells.

作者信息

Matsuoka Satomi, Miyanaga Yukihiro, Yanagida Toshio, Ueda Masahiro

出版信息

Cold Spring Harb Protoc. 2012 Mar 1;2012(3):346-8. doi: 10.1101/pdb.prot068205.

Abstract

Environmental changes result in signaling events at cell membranes. To develop the means to understand these events at the molecular level, it is essential to become familiar with the stochastic nature of signaling molecules in living cells. Using total internal reflection fluorescent microscopy (TIRFM), these signaling events can be directly observed at the single-molecule level. This protocol describes the preparation of an imaging chamber to visualize single molecules in living Dictyostelium cells, which are highly sensitive to chemoattractant stimulation. It also describes treatment of the cells to allow visualization. Chemotactically competent cells are treated with the desired chemical, and the cell suspension is delivered onto coverslips and then overlaid with a thin agarose sheet in preparation for imaging. The cells are typically treated with a fluorescently labeled stimulant or inhibitor. Alternatively, the cells can be stimulated with photoreactive chemicals by using caged compounds. A caged compound is photoactivatable by irradiation with ultraviolet (UV) light, which cleaves a linker conjugating a caging moiety and a chemical. Thus, at a desired moment during recording of the single-molecule images, the concentration of the chemicals can be increased by photolysis of the caged compounds included in the buffer.

摘要

环境变化会导致细胞膜上的信号事件。为了开发在分子水平上理解这些事件的方法,必须熟悉活细胞中信号分子的随机性质。使用全内反射荧光显微镜(TIRFM),可以在单分子水平直接观察这些信号事件。本方案描述了用于可视化对趋化因子刺激高度敏感的活盘基网柄菌细胞中单个分子的成像室的制备方法。它还描述了对细胞进行处理以实现可视化的方法。将具有趋化能力的细胞用所需的化学物质处理,然后将细胞悬液滴加到盖玻片上,再覆盖一层薄琼脂糖片以准备成像。细胞通常用荧光标记的刺激物或抑制剂处理。或者,可以通过使用笼形化合物用光反应性化学物质刺激细胞。笼形化合物可通过紫外线(UV)照射进行光活化,紫外线会切断连接笼形部分和化学物质的连接基团。因此,在单分子图像记录的特定时刻,可以通过光解缓冲液中包含的笼形化合物来提高化学物质的浓度。

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