Multiplexed In Vivo Imaging with Fluorescence Lifetime‐Modulating Tags

Author:

El Hajji Lina1,Lam France2,Avtodeeva Maria1,Benaissa Hela1,Rampon Christine13,Volovitch Michel1,Vriz Sophie13,Gautier Arnaud14ORCID

Affiliation:

1. Sorbonne Université École Normale Supérieure Université PSL CNRS Laboratoire des Biomolécules LBM Paris 75005 France

2. Institut de Biologie Paris Seine plateforme imagerie photonique I2PS (FR3631) Sorbonne Université CNRS Paris 75005 France

3. Université Paris Cité Paris 75006 France

4. Institut Universitaire de France Paris 75006 France

Abstract

AbstractFluorescence lifetime imaging microscopy (FLIM) opens new dimensions for highly multiplexed imaging in live cells and organisms using differences in fluorescence lifetime to distinguish spectrally identical fluorescent probes. Here, a set of fluorescence‐activating and absorption‐shifting tags (FASTs) capable of modulating the fluorescence lifetime of embedded fluorogenic 4‐hydroxybenzylidene rhodanine (HBR) derivatives is described. It is shown that changes in the FAST protein sequence can vary the local environment of the chromophore and lead to significant changes in fluorescence lifetime. These fluorescence lifetime‐modulating tags enable multiplexed imaging of up to three targets in one spectral channel using a single HBR derivative in live cells and live zebrafish larvae. The combination of fluorescence lifetime multiplexing with spectral multiplexing allows to successfully image six targets in live cells, opening great prospects for multicolor fluorescence lifetime multiplexing.

Funder

Fondation pour la Recherche Médicale

H2020 European Research Council

Publisher

Wiley

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