Super-resolution two-photon microscopy via scanning patterned illumination

被引:43
|
作者
Urban, Ben E. [1 ]
Yi, Ji [1 ]
Chen, Siyu [1 ]
Dong, Biqin [1 ]
Zhu, Yongling [2 ]
DeVries, Steven H. [2 ]
Backman, Vadim [1 ]
Zhang, Hao F. [1 ,2 ]
机构
[1] Northwestern Univ, Dept Biomed Engn, Evanston, IL 60208 USA
[2] Northwestern Univ, Dept Ophthalmol, Chicago, IL 60611 USA
来源
PHYSICAL REVIEW E | 2015年 / 91卷 / 04期
基金
美国国家科学基金会;
关键词
STRUCTURED-ILLUMINATION; FLUORESCENCE MICROSCOPY; LATERAL RESOLUTION; AXIAL RESOLUTION; EXCITATION; LIVE; ARCHITECTURE; DYNAMICS; TISSUE; 3D;
D O I
10.1103/PhysRevE.91.042703
中图分类号
O35 [流体力学]; O53 [等离子体物理学];
学科分类号
070204 ; 080103 ; 080704 ;
摘要
We developed two-photon scanning patterned illumination microscopy (2P-SPIM) for super-resolution two-photon imaging. Our approach used a traditional two-photon microscopy setup with temporally modulated excitation to create patterned illumination fields. Combing nine different illuminations and structured illumination reconstruction, super-resolution imaging was achieved in two-photon microscopy. Using 2P-SPIM we achieved a lateral resolution of 141 nm, which represents an improvement by a factor of 1.9 over the corresponding diffraction limit. We further demonstrated super-resolution cellular imaging by 2P-SPIM to image actin cytoskeleton in mammalian cells and three-dimensional imaging in highly scattering retinal tissue.
引用
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页数:6
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