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Correlative microscopy approach for biology using X-ray holography, X-ray scanning diffraction and STED microscopy

机译:使用X射线全息术,X射线扫描衍射和STED显微镜的生物学相关显微镜方法

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We present a correlative microscopy approach for biology based on holographic X-ray imaging, X-ray scanning diffraction, and stimulated emission depletion (STED) microscopy. All modalities are combined into the same synchrotron endstation. In this way, labeled and unlabeled structures in cells are visualized in a complementary manner. We map out the fluorescently labeled actin cytoskeleton in heart tissue cells and superimpose the data with phase maps from X-ray holography. Furthermore, an array of local far-field diffraction patterns is recorded in the regime of small-angle X-ray scattering (scanning SAXS), which can be interpreted in terms of biomolecular shape and spatial correlations of all contributing scattering constituents. We find that principal directions of anisotropic diffraction patterns coincide to a certain degree with the actin fiber directions and that actin stands out in the phase maps from holographic recordings. In situ STED recordings are proposed to formulate models for diffraction data based on co-localization constraints.
机译:我们提出了一种基于全息X射线成像,X射线扫描衍射和受激发射损耗(STED)显微镜的生物学相关显微镜方法。所有形式都组合到同一个同步加速器终端站中。以这种方式,以互补的方式可视化细胞中的标记和未标记的结构。我们绘制了心脏组织细胞中荧光标记的肌动蛋白细胞骨架,并将数据与来自X射线全息术的相位图叠加。此外,在小角度X射线散射(扫描SAXS)状态下记录了一系列局部远场衍射图样,这可以根据生物分子形状和所有贡献性散射成分的空间相关性来解释。我们发现各向异性衍射图样的主要方向与肌动蛋白纤维的方向在一定程度上重合,并且肌动蛋白在全息记录的相位图中脱颖而出。提出了原位STED记录,以基于共定位约束条件为衍射数据建立模型。

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