Fast Optical Sectioning for Widefield Fluorescence Mesoscopy with the Mesolens based on HiLo Microscopy

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作者
Jan Schniete
Aimee Franssen
John Dempster
Trevor J Bushell
William Bradshaw Amos
Gail McConnell
机构
[1] University of Strathclyde,Department of Physics
[2] University of Strathclyde,Strathclyde Institute of Pharmacy and Biomedical Sciences
[3] Cambridge Biomedical Campus,MRC Laboratory of Molecular Biology
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关键词
Mesola; Widefield; Optical Section Thickness; Selective Plane Illumination Microscopy (SPIM); Thin Fluorescent Layer;
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摘要
We present here a fast optical sectioning method for mesoscopy based on HiLo microscopy, which makes possible imaging of specimens of up to 4.4 mm × 3 mm × 3 mm in volume in under 17 hours (estimated for a z-stack comprising 1000 images excluding computation time) with subcellular resolution throughout. Widefield epifluorescence imaging is performed with the Mesolens using a high pixel-number camera capable of sensor-shifting to generate a 259.5 Megapixel image, and we have developed custom software to perform HiLo processing of the very large datasets. Using this method, we obtain comparable sectioning strength to confocal laser scanning microscopy (CLSM), with sections as thin as 6.8 ± 0.2 μm and raw acquisition speed of 1 minute per slice which is up to 30 times faster than CLSM on the full field of view (FOV) of the Mesolens of 4.4 mm with lateral resolution of 0.7 μm and axial resolution of 7 μm. We have applied this HiLo mesoscopy method to image fixed and fluorescently stained hippocampal neuronal specimens and a 5-day old zebrafish larva.
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