Acta Optica Sinica, Volume. 37, Issue 3, 318007(2017)

Light-Sheet Fluorescence Microscopy

Yang Yulong*, Zong Weijian, Wu Runlong, and Chen Liangyi
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  • [in Chinese]
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    In the past two decades, laser scanning confocal microscope has been the standard tool for observing the process of life at cellular and sub-cellular level. The optical sectioning capacity of pinhole-based confocal microscope comes at the price of unwanted excitation of fluorophores out of focal plane and phototoxic damage to biological samples. As a new type of fluorescent microscope, light-sheet fluorescence microscope (LSFM) uses side illumination to conduct surface imaging of the samples directly. As compared to the point-scanning imaging mode, LSFM excels at its imaging speed, which is much higher than that of laser scanning confocal microscope, thus making it possible to study some high-speed fine life activities. Another advantage of the light-sheet fluorescence microscope is that only the sample at the light-sheet is excited and the sample outside the light-sheet is not excited, so there is less phototoxic dosage and we can observe the sample in a longer time scale. The special illumination and imaging mode of the light-sheet fluorescence microscope make it play an irreplaceable role in three-dimensional high-speed imaging of big biological samples. The history and research status of light-sheet fluorescence microscope are reviewed with the purpose of providing a personal perspective of current situation and future direction of LSFM.

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    Yang Yulong, Zong Weijian, Wu Runlong, Chen Liangyi. Light-Sheet Fluorescence Microscopy[J]. Acta Optica Sinica, 2017, 37(3): 318007

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    Paper Information

    Received: Dec. 6, 2016

    Accepted: --

    Published Online: Mar. 8, 2017

    The Author Email: Yulong Yang (yangyulong@pku.edu.cn)

    DOI:10.3788/aos201737.0318007

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