A robust and versatile platform for image scanning microscopy enabling super-resolution FLIM.

Marco CastelloGiorgio Tortarolo Mauro ButtafavaTakahiro DeguchiFederica VillaSami KohoLuca PesceMichele OnetoSimone PelicciLuca LanzanóPaolo BianchiniColin J R SheppardAlberto Diaspro Alberto Tosi Giuseppe Vicidomini

Published in: Nature methods (2019)

Image scanning microscopy (ISM) can improve the effective spatial resolution of confocal microscopy to its theoretical limit. However, current implementations are not robust or versatile, and are incompatible with fluorescence lifetime imaging (FLIM). We describe an implementation of ISM based on a single-photon detector array that enables super-resolution FLIM and improves multicolor, live-cell and in-depth imaging, thereby paving the way for a massive transition from confocal microscopy to ISM.

Keyphrases

high resolution
single molecule
high throughput
deep learning
mass spectrometry
high speed
primary care
healthcare
electron microscopy
magnetic resonance imaging
magnetic resonance
photodynamic therapy
quantum dots
image quality