Three-dimensional laser microsurgery in light-sheet based microscopy (SPIM)

被引:45
作者
Engelbrecht, Christoph J.
Greger, Klaus
Reynaud, Emmanuel G.
Krzic, Uros
Colombelli, Julien
Stelzer, Ernst H. K.
机构
[1] EMBL Heidelberg, Light Microscopy Grp, Cell Biol & Biophys Unit, D-69117 Heidelberg, Germany
[2] Univ Zurich, Dept Neurophysiol, Brain Res Inst, CH-8057 Zurich, Switzerland
[3] Swiss Fed Inst Technol, CH-8057 Zurich, Switzerland
来源
OPTICS EXPRESS | 2007年 / 15卷 / 10期
关键词
D O I
10.1364/OE.15.006420
中图分类号
O43 [光学];
学科分类号
070207 ; 0803 ;
摘要
Advances in the life sciences rely on the ability to observe dynamic processes in live systems and in environments that mimic in-vivo situations. Therefore, new methodological developments have to provide environments that resemble physiologically and clinically relevant conditions as closely as possible. In this work, plasma-induced laser nanosurgery for three-dimensional sample manipulation and sample perturbation is combined with optically sectioning light-sheet based fluorescence microscopy (SPIM) and applied to three-dimensional biological model systems. This means: a) working with a biological system that is not confined to essentially two dimensions like cell cultures on cover glasses, b) gaining intrinsic optical sectioning capabilities by an efficient three-dimensional fluorescence imaging system, and c) using arbitrarily-shaped three-dimensional ablation-patterns by a plasma-induced laser ablation system that prevent damage to surrounding tissues. Spatial levels in our biological applications range from sub-microns during delicate ablation of single microtubules over the confined disruption of cell membranes in an MDCK-cyst to the macroscopic cutting of a millimeter-sized Zebrafish caudal fin with arbitrary three-dimensional ablation patterns. Dynamic processes like laser-induced hemocyte migration can be studied with our SPIM-microscalpel in intact, live embryos. (C) 2007 Optical Society of America
引用
收藏
页码:6420 / 6430
页数:11
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