Integrated 3D macro-trapping and light-sheet imaging system

被引:0
|
作者
Yang, Zhengyi [1 ]
Piksarv, Peeter [1 ,2 ]
Ferrier, David E. K. [3 ]
Gunn-Moore, Frank J. [4 ]
Dholakia, Kishan [1 ]
机构
[1] Univ St Andrews, Sch Phys & Astron, SUPA, St Andrews KY16 9SS, Fife, Scotland
[2] Univ Tartu, Inst Phys, EE-50411 Tartu, Estonia
[3] Univ St Andrews, Sch Biol, Scottish Oceans Inst, Gatty Marine Lab, St Andrews KY16 8LB, Fife, Scotland
[4] Univ St Andrews, Sch Biol, St Andrews KY16 9FT, Fife, Scotland
关键词
Light sheet imaging; dual-beam trap; optical trapping; counter-propagating trap; openSPIM; Spirobranchus lamarcki larva; OPTICAL TRAPS; MICROSCOPY; EMBRYOS; DEEP;
D O I
10.1117/12.2186399
中图分类号
O43 [光学];
学科分类号
070207 ; 0803 ;
摘要
Biological research requires high-speed and low-damage imaging techniques for live specimens in areas such as development study in embryos. Light sheet microscopy provides fast imaging speed whilst keeps the photo-damage and photo-blenching to minimum. Conventional sample embedding methods in light sheet imaging involves using agent such as agarose which potentially affects the behavior and the develop pattern of the specimens. Here we demonstrate integrating dual-beam trapping method into light sheet imaging system to confine and translate the specimen whilst light sheet images are taken. Tobacco plant cells as well as Spirobranchus lamarcki larva were trapped solely with optical force and sectional images were acquired. This now approach has the potential to extend the applications of light sheet imaging significantly.
引用
收藏
页数:6
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