KEYWORDS: Fluorescence lifetime imaging, Microscopes, Confocal microscopy, Luminescence, Live cell imaging, Surface plasmons, In vivo imaging, Single photon, Resonance energy transfer, Imaging systems
We report the development of a novel confocal line-scanning microscope capable of acquiring video-frame rate TCSPC-based FLIM. The system consists of a one-dimensional laser beam, which is optically conjugated to a 1024×16 single photon avalanche diode(SPAD) based line-imaging CMOS(1), with 23.78 μm pixel pitch at 49.31% fill factor. Incorporation of on-chip histogramming on the line-sensor facilitates the acquisition of up to 16.5 Giga-photon counts/s, enabling operation 66 times faster than our previously reported bespoke high speed FLIM platforms. We will demonstrate its use in live-cell imaging investigating the roles that PAK proteins play in regulation of cytoskeletal dynamics.
Precisely characterising and quantifying interactions between tumour cells and their environment to understand metastatic mechanisms requires a multi-dimensional, high-speed imaging system. To this end, we report on the development of a compressive full spectrum fluorescence lifetime microscope that exploits a novel SPAD line sensor and a DMD to enable monitoring of dynamic sub-cellular interactions. At no cost to its temporal performance, the hyperspectral nature of the system helps to improve unmixing and, crucially, can detect the small spectral changes in the emission of fluorescent probes and intrinsic fluorophores that can occur in complex environments.
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