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csiLSFM combines light-sheet fluorescence microscopy and coherent structured illumination for a lateral resolution below 100 nm

机译:csiLSFM结合了光片荧光显微镜和相干结构照明横向分辨率低于100 nm

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摘要

Light-sheet-based fluorescence microscopy (LSFM) features optical sectioning in the excitation process. It minimizes fluorophore bleaching as well as phototoxic effects and provides a true axial resolution. The detection path resembles properties of conventional fluorescence microscopy. Structured illumination microscopy (SIM) is attractive for superresolution because of its moderate excitation intensity, high acquisition speed, and compatibility with all fluorophores. We introduce SIM to LSFM because the combination pushes the lateral resolution to the physical limit of linear SIM. The instrument requires three objective lenses and relies on methods to control two counterpropagating coherent light sheets that generate excitation patterns in the focal plane of the detection lens. SIM patterns with the finest line spacing in the far field become available along multiple orientations. Flexible control of rotation, frequency, and phase shift of the perfectly modulated light sheet are demonstrated. Images of beads prove a near-isotropic lateral resolution of sub-100 nm. Images of yeast endoplasmic reticulum show that coherent structured illumination (csi) LSFM performs with physiologically relevant specimens.
机译:基于光片的荧光显微镜(LSFM)在激发过程中具有光学切片功能。它最大程度地减少了荧光团的漂白和光毒作用,并提供了真正的轴向分辨率。检测路径类似于常规荧光显微镜的特性。结构照明显微镜(SIM)具有超强的吸引力,因为它具有中等强度的激发强度,高采集速度以及与所有荧光团的相容性。我们将SIM引入LSFM是因为这种组合将横向分辨率提高到了线性SIM的物理极限。该仪器需要三个物镜,并依赖于控制两个反向传播的相干光片的方法,该相干光片在检测透镜的焦平面上生成激发图案。可以在多个方向上使用在远场中具有最佳行距的SIM卡图案。演示了灵活控制完美调制的光片的旋转,频率和相移。珠子的图像证明了接近100 nm的各向同性横向分辨率。酵母内质网图像显示相干结构照度(csi)LSFM对生理相关标本起作用。

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