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Scanning superlens microscopy for non-invasive large field-of-view visible light nanoscale imaging

机译:扫描超透镜显微镜用于无创大视野可见光纳米级成像

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摘要

Nanoscale correlation of structural information acquisition with specific-molecule identification provides new insight for studying rare subcellular events. To achieve this correlation, scanning electron microscopy has been combined with super-resolution fluorescent microscopy, despite its destructivity when acquiring biological structure information. Here we propose time-efficient non-invasive microsphere-based scanning superlens microscopy that enables the large-area observation of live-cell morphology or sub-membrane structures with sub-diffraction-limited resolution and is demonstrated by observing biological and non-biological objects. This microscopy operates in both non-invasive and contact modes with ∼200 times the acquisition efficiency of atomic force microscopy, which is achieved by replacing the point of an atomic force microscope tip with an imaging area of microspheres and stitching the areas recorded during scanning, enabling sub-diffraction-limited resolution. Our method marks a possible path to non-invasive cell imaging and simultaneous tracking of specific molecules with nanoscale resolution, facilitating the study of subcellular events over a total cell period.
机译:结构信息获取与特定分子识别的纳米级关联为研究罕见的亚细胞事件提供了新的见识。为了实现这种关联,尽管在获取生物结构信息时具有破坏性,但扫描电子显微镜已与超分辨率荧光显微镜相结合。在这里,我们提出了一种基于时间的非侵入性基于微球的扫描超透镜显微镜,该显微镜能够以亚衍射极限分辨率大面积观察活细胞形态或亚膜结构,并通过观察生物和非生物物体来证明。该显微镜可在非侵入式和接触式两种模式下运行,其获取效率是原子力显微镜的200倍左右,这是通过用微球的成像区域代替原子力显微镜尖端的点并缝合扫描过程中记录的区域来实现的,启用亚衍射极限分辨率。我们的方法标志着非侵入性细胞成像和同时追踪具有纳米级分辨率的特定分子的可能路径,从而有助于研究整个细胞周期内的亚细胞事件。

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