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Photoimprint Photoacoustic Microscopy for Three-Dimensional Label-Free Subdiffraction Imaging

机译:用于三维无标记亚衍射成像的光压印光声显微镜

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摘要

Subdiffraction optical microscopy allows the imaging of cellular and subcellular structures with a resolution finer than the diffraction limit. Here, combining the absorption-based photoacoustic effect and intensity-dependent photobleaching effect, we demonstrate a simple method for subdiffraction photoacoustic imaging of both fluorescent and nonfluorescent samples. Our method is based on a double-excitation process, where the first excitation pulse partially and inhomogeneously bleaches the molecules in the diffraction-limited excitation volume, thus biasing the signal contributions from a second excitation pulse striking the same region. The differential signal between the two excitations preserves the signal contribution mostly from the center of the excitation volume, and dramatically sharpens the lateral resolution. Moreover, due to the nonlinear nature of the signal, our method offers an inherent optical sectioning capability, which is lacking in conventional photoacoustic microscopy. By scanning the excitation beam, we performed three-dimensional subdiffraction imaging of varied fluorescent and nonfluorescent species. As any molecules have absorption, this technique has the potential to enable label-free subdiffraction imaging, and can be transferred to other optical imaging modalities or combined with other subdiffraction methods.
机译:亚衍射光学显微镜可以对细胞和亚细胞结构进行成像,其分辨率比衍射极限还小。在这里,结合基于吸收的光声效应和强度相关的光漂白效应,我们证明了用于荧光和非荧光样品亚衍射光声成像的简单方法。我们的方法基于双激发过程,其中第一激发脉冲部分地和不均匀地漂白了受衍射限制的激发体积中的分子,从而偏置了来自第二次激发脉冲的相同区域的信号贡献。两次激发之间的差分信号主要保留了激发体积中心的信号贡献,并显着提高了横向分辨率。此外,由于信号的非线性特性,我们的方法提供了固有的光学切片功能,这是常规光声显微镜所没有的。通过扫描激发光束,我们对各种荧光和非荧光物质进行了三维亚衍射成像。由于任何分子都具有吸收作用,因此该技术具有实现无标记亚衍射成像的潜力,并且可以转移到其他光学成像模态或与其他亚衍射方法结合使用。

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