Two-photon instant structured illumination microscopy improves the depth penetration of super-resolution imaging in thick scattering samples

被引:97
|
作者
Winter, Peter W. [1 ]
York, Andrew G. [1 ]
Nogare, Damian Dalle [2 ]
Ingaramo, Maria [3 ]
Christensen, Ryan [1 ]
Chitnis, Ajay [2 ]
Patterson, George H. [3 ]
Shroff, Hari [1 ]
机构
[1] Natl Inst Biomed Imaging & Bioengn, Sect High Resolut Opt Imaging, NIH, Bethesda, MD 20892 USA
[2] Eunice Kennedy Shriver Natl Inst Child Hlth & Hum, Sect Neural Dev Dynam, NIH, Bethesda, MD 20892 USA
[3] Natl Inst Biomed Imaging & Bioengn, Sect Biophoton, NIH, Bethesda, MD 20892 USA
来源
OPTICA | 2014年 / 1卷 / 03期
关键词
FLUORESCENCE MICROSCOPY; ADAPTIVE OPTICS; MOUSE-BRAIN; RESOLUTION; LIVE; 3D; CELLS; NANOSCALE;
D O I
10.1364/OPTICA.1.000181
中图分类号
O43 [光学];
学科分类号
070207 ; 0803 ;
摘要
Fluorescence imaging methods that achieve spatial resolution beyond the diffraction limit (super-resolution) are of great interest in biology. We describe a super-resolution method that combines two-photon excitation with structured illumination microscopy (SIM), enabling three-dimensional interrogation of live organisms with similar to 150 nm lateral and similar to 400 nm axial resolution, at frame rates of similar to 1 Hz. By performing optical rather than digital processing operations to improve resolution, our microscope permits super-resolution imaging with no additional cost in acquisition time or phototoxicity relative to the pointscanning two-photon microscope upon which it is based. Our method provides better depth penetration and inherent optical sectioning than all previously reported super-resolution SIM implementations, enabling super-resolution imaging at depths exceeding 100 mu m from the coverslip surface. The capability of our system for interrogating thick live specimens at high resolution is demonstrated by imaging whole nematode embryos and larvae, and tissues and organs inside zebrafish embryos.
引用
收藏
页码:181 / 191
页数:11
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