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10 April 1996 Fluorescence lifetime imaging in confocal microscopy: signal-to-noise considerations
Kjell Carlsson
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Proceedings Volume 2655, Three-Dimensional Microscopy: Image Acquisition and Processing III; (1996) https://doi.org/10.1117/12.237461
Event: Electronic Imaging: Science and Technology, 1996, San Jose, CA, United States
Abstract
By utilizing lifetime information, in addition to spectral properties, new and interesting possibilities can be realized in confocal fluorescence microscopy. In combination with the previously described Intensity-modulated Multiple-beam Scanning (IMS) technique it is possible to strongly increase the number of fluorophores that can be simultaneously and independently recorded. Another possibility is to detect, simultaneously, changes in the lifetimes of multiple fluorophores caused by changes in the chemical environment such as pH or ion concentration. A factor that critically determines the usefulness of lifetime information is the signal-to-noise ratio (SNR) that can be attained. This paper presents a theoretical investigation of the SNR when using the IMS in combination lifetime measurements. It is found that when increasing the number of simultaneously detected fluorophores, it is important to select fluorophores with widely different lifetimes. For lifetime measurements the precision can be expressed in terms of the number of detected photons.
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Kjell Carlsson "Fluorescence lifetime imaging in confocal microscopy: signal-to-noise considerations", Proc. SPIE 2655, Three-Dimensional Microscopy: Image Acquisition and Processing III, (10 April 1996); https://doi.org/10.1117/12.237461
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KEYWORDS
Signal to noise ratio
Amplifiers
Confocal microscopy
Photons
Modulation
Ions
Fluorescence lifetime imaging
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