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Simultaneous confocal lifetime imaging of multiple fluorophores using the intensity-modulated multiple-wavelength scanning (IMS) technique
Authors:Carlsson,&   Liljeborg
Affiliation:Department of Biomedical and X-ray Physics,;Department of Geodesy and Photogrammetry, The Royal Institute of Technology, SE-100 44 Stockholm, Sweden,;Department of Neuroscience, Karolinska Institute, SE-171 77 Stockholm, Sweden
Abstract:We demonstrate the simultaneous recording of confocal lifetime images of multiple fluorophores. The confocal microscope used in the study combines intensity-modulated laser illumination, lock-in detection and spectral separation of the fluorescent light. A theoretical investigation is presented that describes how the signal-to-noise ratio (SNR) depends on various factors such as modulation frequency, degree of modulation and number of detected photons. Theory predicts that, compared with ordinary intensity images, lifetime images will have a SNR that is, at best, approximately four times lower. Experimental results are presented that confirm this prediction.
Keywords:Confocal microscopy    fluorescence lifetime imaging    signal-to-noise ratio
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