Confocal line scanning of a Bessel beam for fast 3D Imaging

被引:22
|
作者
Zhang, P. [1 ]
Phipps, M. E. [1 ]
Goodwin, P. M. [1 ]
Werner, J. H. [1 ]
机构
[1] Los Alamos Natl Lab, Ctr Integrated Nanotechnol, Los Alamos, NM 87545 USA
关键词
LIGHT-SHEET MICROSCOPY; SINGLE-MOLECULE LOCALIZATION; FLUORESCENCE MICROSCOPY; PLANE ILLUMINATION; THICK MEDIA; EXCITATION; CELLS;
D O I
10.1364/OL.39.003682
中图分类号
O43 [光学];
学科分类号
070207 ; 0803 ;
摘要
We have developed a light-sheet illumination microscope that can perform fast 3D imaging of transparent biological samples with inexpensive visible lasers and a single galvo mirror (GM). The light-sheet is created by raster scanning a Bessel beam with a GM, with this same GM also being used to rescan the fluorescence across a chip of a camera to construct an image in real time. A slit is used to reject out-of-focus fluorescence such that the image formed in real time has minimal contribution from the sidelobes of the Bessel beam. Compared with two-photon Bessel beam excitation or other confocal line-scanning approaches, our method is of lower cost, is simpler, and does not require calibration and synchronization of multiple GMs. We demonstrated the optical sectioning and out-of-focus background rejection capabilities of this microscope by imaging fluorescently labeled actin filaments in fixed 3T3 cells. (C) 2014 Optical Society of America
引用
收藏
页码:3682 / 3685
页数:4
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