ANATOMICAL AND FUNCTIONAL IMAGING OF NEURONS USING 2-PHOTON LASER-SCANNING MICROSCOPY

被引:272
作者
DENK, W
DELANEY, KR
GELPERIN, A
KLEINFELD, D
STROWBRIDGE, BW
TANK, DW
YUSTE, R
机构
[1] Biological Computation Research Department, AT and T Bell Laboratories, Murray Hill
关键词
MICROSCOPY; 2-PHOTON LASER SCANNING; LIGHT SCATTERING; PHOTOTOXICITY; RECEPTOR; NEUROTRANSMITTER;
D O I
10.1016/0165-0270(94)90189-9
中图分类号
Q5 [生物化学];
学科分类号
071010 ; 081704 ;
摘要
Light scattering by brain tissue and phototoxicity are major obstacles to the use of high-resolution optical imaging and photo-activation ('uncaging') of bioactive compounds from inactive ('caged') precursors in intact and semi-intact nervous systems. Optical methods based on 2-photon excitation promise to reduce these obstacles (Denk, 1994; Denk et al., 1990, 1994). Here we show a range of imaging modes based on 2-photon laser scanning microscopy (TPLSM) as applicable to problems in neuroscience. Fluorescence images were taken of neurons labeled with ion-sensitive and voltage-sensitive dyes in invertebrate ganglia, mammalian brain slices, and from the intact mammalian brain. Scanning photochemical images with whole-cell current detection (Denk, 1994) show how the distribution of neurotransmitter receptors on the surface of specific cells can be mapped. All images show strong optical sectioning and usable images can be obtained at depths greater than 100 mu m below the surface of the preparation.
引用
收藏
页码:151 / 162
页数:12
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