Abstract
Fluorescence lifetime imaging is an important tool in bioimaging that allows one to detect subtle changes in cell dynamics and their environment. Most time-domain approaches currently involve scanning a single illumination point across the sample, which can make imaging dynamic scenes challenging, while single-shot “rapid lifetime determination” can suffer from large uncertainties when the lifetime is not appropriately sampled. Here, we propose a time-folded fluorescence lifetime imaging microscopy (TFFLIM) approach, whereby a time-folding cavity provides multiple spatially sheared replicas of the lifetime, each shifted temporally with respect to a fixed time gate. This provides a robust, single-shot FLIM approach that we experimentally validate across a broad lifetime range on fluorescent beads and Convallaria samples.
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CITATION STYLE
Kapitany, V., Zickus, V., Fatima, A., Carles, G., & Faccio, D. (2023). Single-shot time-folded fluorescence lifetime imaging. Proceedings of the National Academy of Sciences of the United States of America, 120(16). https://doi.org/10.1073/pnas.2214617120
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