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Mapping Pixel Dissimilarity in Wide-Field Super-Resolution Fluorescence Microscopy

机译:广域超高分辨率荧光显微镜中的像素差异映射

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Recent advances in fluorescence bioimaging with single-molecule sensitivity have relied on the analysis and visualization of single-molecule data obtained on smart fluorophores. We describe an alternative method to enhance the information content of densely labeled fluorescence images. Visualization is improved by representing pixels as the dissimilarities of the fluctuations of the fluorescence signals, with the dissimilarity being taken to the mean of the signals over all the pixels. Mapping pixel dissimilarity (Mappix) results in signal and information enhancement of the output images. In addition, the spatial distribution of the fluorescence brightness of the original image is not skewed. This allows large differences of molecular brightness to be handled which turns out to be critical to the fidelity of the final image. In this work, we provide testing of the Mappix approach with both simulated and real data. The results obtained on HEK cells expressing Dronpa photoswitchable fluorescent protein show that, for densely labeled samples, improvement can be obtained on fluorescence images allowing the observation of structural information. Despite some limitations, comparison to state of art methods reveals that Mappix can be very useful for biological imaging applications.
机译:具有单分子敏感性的荧光生物成像的最新进展依赖于在智能荧光团上获得的单分子数据的分析和可视化。我们描述了一种替代方法来增强密集标记的荧光图像的信息内容。通过将像素表示为荧光信号波动的不相似性来改善可视化效果,其中不相似性被视为所有像素上信号的平均值。映射像素差异(Mappix)会增强输出图像的信号和信息。另外,原始图像的荧光亮度的空间分布不偏斜。这允许处理较大的分子亮度差异,这对于最终图像的保真度至关重要。在这项工作中,我们将使用模拟数据和真实数据对Mappix方法进行测试。在表达Dronpa光可切换荧光蛋白的HEK细胞上获得的结果表明,对于密集标记的样品,荧光图像可以得到改善,从而可以观察结构信息。尽管有一些限制,但与现有技术方法进行比较发现,Mappix对于生物成像应用可能非常有用。

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