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具有时空结构照明的共聚焦激光扫描显微镜。

Confocal laser scanning microscopy with spatiotemporal structured illumination.

作者信息

Gao Peng, Nienhaus G Ulrich

出版信息

Opt Lett. 2016 Mar 15;41(6):1193-6. doi: 10.1364/OL.41.001193.

Abstract

Confocal laser scanning microscopy (CLSM), which is widely utilized in the biological and biomedical sciences, is limited in spatial resolution due to diffraction to about half the light wavelength. Here we have combined structured illumination with CLSM to enhance its spatial resolution. To this end, we have used a spatial light modulator (SLM) to generate fringe patterns of different orientations and phase shifts in the excitation spot without any mechanical movement. We have achieved 1.8 and 1.7 times enhanced lateral and axial resolutions, respectively, by synthesizing the object spectrum along different illumination directions. This technique is thus a promising tool for high-resolution morphological or fluorescence imaging, especially in deep tissue.

摘要

共聚焦激光扫描显微镜(CLSM)在生物和生物医学科学中被广泛应用,但由于衍射,其空间分辨率限制在约光波长的一半左右。在此,我们将结构照明与CLSM相结合以提高其空间分辨率。为此,我们使用空间光调制器(SLM)在激发光斑中生成不同方向和相移的条纹图案,而无需任何机械移动。通过沿不同照明方向合成物体光谱,我们分别实现了横向分辨率提高1.8倍和轴向分辨率提高1.7倍。因此,这项技术是用于高分辨率形态学或荧光成像的有前途的工具,特别是在深部组织中。

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