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Axial plane single-molecule super-resolution microscopy of whole cells

机译:全细胞轴平面单分子超分辨显微镜

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摘要

Fluorescence nanoscopy has become an indispensable tool for studying organelle structures, protein dynamics, and interactions in biological sciences. Single-molecule localization microscopy can now routinely achieve 10–50 nm resolution through fluorescently labeled specimens in lateral optical sections. However, visualizing structures organized along the axial direction demands scanning and imaging each of the lateral imaging planes with fine intervals throughout the whole cell. This iterative process suffers from photobleaching of tagged probes, is susceptible to alignment artifacts and also limits the imaging speed. Here, we focused on the axial plane super-resolution imaging which integrated the single-objective light-sheet illumination and axial plane optical imaging with single-molecule localization technique to resolve nanoscale cellular architectures along the axial (or depth) dimension without scanning. We demonstrated that this method is compatible with DNA points accumulation for imaging in nanoscale topography (DNA-PAINT) and exchange-PAINT by virtue of its light-sheet illumination, allowing multiplexed super-resolution imaging throughout the depth of whole cells. We further demonstrated this proposed system by resolving the axial distributions of intracellular organelles such as microtubules, mitochondria, and nuclear pore complexes in both COS-7 cells and glioblastoma patient-derived tumor cells.
机译:荧光纳米显微镜已成为研究生物科学中细胞器结构,蛋白质动力学和相互作用的必不可少的工具。单分子定位显微镜现在可以通过侧向光学切片中的荧光标记标本常规获得10–50 nm的分辨率。然而,沿轴向组织的可视化结构需要在整个细胞内以精细间隔扫描和成像每个横向成像平面。该迭代过程遭受标记探针的光漂白的影响,易受对准伪影的影响,并且还限制了成像速度。在这里,我们着重研究轴向平面超分辨率成像技术,该技术将单目标光片照明和轴向平面光学成像技术与单分子定位技术相结合,无需扫描即可沿轴向(或深度)方向解析纳米尺度的细胞结构。我们证明了这种方法与DNA点累积兼容,因为它具有光片照明功能,可以在纳米级地形(DNA-PAINT)和exchange-PAINT中成像,从而可以在整个细胞的整个深度进行多重超分辨率成像。我们通过解决COS-7细胞和成胶质细胞瘤患者来源的肿瘤细胞中细胞内细胞器(例如微管,线粒体和核孔复合体)的轴向分布,进一步证明了该提议的系统。

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