High-throughput isotropic mapping of whole mouse brain using multi-view light-sheet microscopy

被引:0
|
作者
Nie, Jun [1 ]
Li, Yusha [2 ]
Zhao, Fang [1 ]
Ping, Junyu [1 ]
Liu, Sa [1 ]
Yu, Tingting [2 ]
Zhu, Dan [2 ]
Fei, Peng [1 ,2 ]
机构
[1] Huazhong Univ Sci & Technol, Sch Opt & Elect Informat, Wuhan 430074, Hubei, Peoples R China
[2] Huazhong Univ Sci & Technol, Britton Chance Ctr Biomed Photon, Wuhan Natl Lab Optoelect, Wuhan 430074, Hubei, Peoples R China
来源
关键词
Light-sheet microscopy; whole-brain imaging; multi-view deconvolution; RESOLUTION; ULTRAMICROSCOPY; RECONSTRUCTION; POPULATIONS; EMBRYOS;
D O I
10.1117/12.2295273
中图分类号
R445 [影像诊断学];
学科分类号
100207 ;
摘要
Light-sheet fluorescence microscopy (LSFM) uses an additional laser-sheet to illuminate selective planes of the sample, thereby enabling three-dimensional imaging at high spatial-temporal resolution. These advantages make LSFM a promising tool for high-quality brain visualization. However, even by the use of LSFM, the spatial resolution remains insufficient to resolve the neural structures across a mesoscale whole mouse brain in three dimensions. At the same time, the thick-tissue scattering prevents a clear observation from the deep of brain. Here we use multi-view LSFM strategy to solve this challenge, surpassing the resolution limit of standard light-sheet microscope under a large field-of-view (FOV). As demonstrated by the imaging of optically-cleared mouse brain labelled with thyl-GFP, we achieve a brain-wide, isotropic cellular resolution of similar to 3 mu m. Besides the resolution enhancement, multi-view braining imaging can also recover complete signals from deep tissue scattering and attenuation. The identification of long distance neural projections across encephalic regions can be identified and annotated as a result.
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页数:6
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