Name:SPIM microscope
Model:Lightsheet Z.1
Description:Light sheet fluorescence microscopy or LSFM splits fluorescence excitation and detection into two separate light paths, with the axis of illumination perpendicular to the detection axis. That means you illuminate a single thin section of your sample at one time, generating an inherent optical section by exciting only fluorescence from the in-focus plane. No pinhole or image processing is required for light sheet microscopy. Light from the in-focus plane is collected on the pixels of a camera, rather than pixel by pixel as, for example, in confocal or other laser scanning microscopy approaches. Parallelization of the image collection on a camera-based detector lets you collect images faster and with less excitation light than you would with many other microscope techniques.
Responsible person:Tomasz Węgierski (ext. 763)

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