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首页> 外文期刊>Biomedical Optics Express >Enhancement of lateral resolution and optical sectioning capability of two-photon fluorescence microscopy by combining temporal-focusing with structured illumination
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Enhancement of lateral resolution and optical sectioning capability of two-photon fluorescence microscopy by combining temporal-focusing with structured illumination

机译:通过将时间聚焦与结构化照明相结合来提高双光子荧光显微镜的横向分辨率和光学切片能力

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摘要

We demonstrate super-resolution imaging with background fluorescence rejection by interferometric temporal focusing microscopy, in which temporal focusing is combined with structured illumination. The lateral resolution and the optical sectioning capability are simultaneously improved by factors of 1.6 and 1.4, respectively, compared to conventional temporal focusing microscopy. Fluorescent beads (200 nm diameter) that are difficult to distinguish from the background fluorescence in conventional temporal focusing microscopy, are clearly visualized by interferometric temporal focusing microscopy.
机译:我们展示了通过干涉式时间聚焦显微镜在背景荧光抑制下的超分辨率成像,其中时间聚焦与结构化照明相结合。与传统的时间聚焦显微镜相比,横向分辨率和光学切片能力分别提高了1.6倍和1.4倍。在传统的时间聚焦显微镜中难以与背景荧光区分开的荧光珠(直径200 nm)可以通过干涉式时间聚焦显微镜清楚地看到。

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