Flow cytometry and integrated imaging

被引:12
|
作者
Kachel, V [1 ]
Wietzorrek, J [1 ]
机构
[1] Max Planck Inst Biochem, D-82152 Martinsried, Germany
关键词
flow cytometry; imaging; flash illumination; nanolite; LED-flash;
D O I
10.3989/scimar.2000.64n2247
中图分类号
Q17 [水生生物学];
学科分类号
071004 ;
摘要
It is a serious problem to relate the results of a flow cytometric analysis of a marine sample to different species. Images of particles selectively triggered by the flow cytometric analysis and picked out from the flowing stream give a valuable additional information on the analyzed organisms. The technical principles and problems of triggered imaging in flow are discussed, as well as the positioning of the particles in the plane of focus, freezing the motion of the quickly moving objects and what kinds of light sources are suitable for pulsed illumination. The images have to be stored either by film or electronically. The features of camera targets and the memory requirements for storing the image data and the conditions for the triggering device are shown. A brief explanation of the features of three realized flow cytometric imaging (FCI) systems is given: the Macro Flow Planktometer built within the EUROMAR MAROPT project, the Imaging Module of the European Plankton Analysis System, supported by the MAST II EurOPA project and the most recently developed FLUVO VI universal flow cytometer including HBO 100- and laser excitation for fluorescence and scatter, Coulter sizing as well as bright field and and phase contrast FCI.
引用
收藏
页码:247 / 254
页数:8
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