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Photoactivatable mCherry for high-resolution two-color fluorescence microscopy

机译:可光活化的mCherry用于高分辨率双色荧光显微镜

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摘要

The reliance of modern microscopy techniques on photoactivatable fluorescent proteins prompted development of mCherry variants that are initially dark but become red fluorescent after violet-light irradiation. Using ensemble and single-molecule characteristics as selection criteria, we developed PAmCherry1 with excitation/emission maxima at 564/595 nm. Compared to other monomeric red photoactivatable proteins, it has faster maturation, better pH stability, faster photoactivation, higher photoactivation contrast and better photostability. Lack of green fluorescence and single-molecule behavior make monomeric PAmCherry1 a preferred tag for two-color diffraction-limited photoactivation imaging and for super-resolution techniques such as one- and two-color photoactivated localization microscopy (PALM). We performed PALM imaging using PAmCherry1-tagged transferrin receptor expressed alone or with photoactivatable GFP–tagged clathrin light chain. Pair correlation and cluster analyses of the resulting PALM images identified ≤200 nm clusters of transferrin receptor and clathrin light chain at ≤25 nm resolution and confirmed the utility of PAmCherry1 as an intracellular probe.
机译:现代显微镜技术对可光激活的荧光蛋白的依赖促使了mCherry变体的发展,这些变体最初是黑暗的,但在紫光照射后变成红色荧光。使用集合和单分子特征作为选择标准,我们开发了最大激发/发射在564/595 nm的PAmCherry1。与其他单体红色可光活化蛋白质相比,它具有更快的成熟度,更好的pH稳定性,更快的光活化,更高的光活化对比度和更好的光稳定性。缺少绿色荧光和单分子行为使单体PAmCherry1成为用于两色衍射限制光活化成像和超分辨率技术(例如一色和两色光活化定位显微镜(PALM))的首选标签。我们使用单独表达的PAmCherry1标签的转铁蛋白受体或带有光激活的GFP标签的网格蛋白轻链进行了PALM成像。对所得PALM图像的配对相关性和聚类分析确定了在≤25 nm分辨率下≤200 nm的运铁蛋白受体和网格蛋白轻链簇,并确认了PAmCherry1作为细胞内探针的实用性。

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