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research article

Light- field tomographic fluorescence lifetime imaging microscopy

Ma, Yayao
•
Park, Jongchan
•
Huang, Lu-Zhe
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October 1, 2024
Proceedings Of The National Academy Of Sciences Of The United States Of America (PNAS)

Fluorescence lifetime imaging microscopy (FLIM) is a powerful imaging technique that enables the visualization of biological samples at the molecular level by measuring the fluorescence decay rate of fluorescent probes. This provides critical information about molecular interactions, environmental changes, and localization within biological systems. However, creating high- resolution lifetime maps using conventional FLIM systems can be challenging, as it often requires extensive scanning that can significantly lengthen acquisition times. This issue is further compounded in three- dimensional (3D) imaging because it demands additional scanning along the depth axis. To tackle this challenge, we developed a computational imaging technique called light- field tomographic FLIM (LIFT- FLIM). Our approach allows for the acquisition of volumetric fluorescence lifetime images in a highly data- efficient manner, significantly reducing the number of scanning steps required compared to conventional point- scanning or line- scanning FLIM imagers. Moreover, LIFT-FLIM enables the measurement of high- dimensional data using low- dimensional detectors, which are typically low cost and feature a higher temporal bandwidth. We demonstrated LIFT-FLIM using a linear single- photon avalanche diode array on various biological systems, showcasing unparalleled single- photon detection sensitivity. Additionally, we expanded the functionality of our method to spectral FLIM and demonstrated its application in high- content multiplexed imaging of lung organoids. LIFT-FLIM has the potential to open up broad avenues in both basic and translational biomedical research.

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Type
research article
DOI
10.1073/pnas.2402556121
Web of Science ID

WOS:001348579900002

PubMed ID

39320920

Author(s)
Ma, Yayao

University of California System

Park, Jongchan

University of California System

Huang, Lu-Zhe

University of California System

Sen, C.
Burri, Samuel  

École Polytechnique Fédérale de Lausanne

Bruschini, Claudio  

École Polytechnique Fédérale de Lausanne

Yang, Xilin

University of California System

Cui, Qi

University of California System

Cameron, R. B.

University of California System

Fishbein, Gregory A.

University of California System

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Date Issued

2024-10-01

Publisher

National Academy of Sciences

Published in
Proceedings Of The National Academy Of Sciences Of The United States Of America (PNAS)
Volume

121

Issue

40

Article Number

e2402556121

Subjects

fluorescence lifetime imaging microscopy

•

3D imaging

•

light field imaging

•

https

•

//doi.org/10.1073/pnas.2402556121

Editorial or Peer reviewed

REVIEWED

Written at

EPFL

EPFL units
AQUA  
FunderFunding(s)Grant NumberGrant URL

United States Department of Health & Human Services

R01HL165318;RF1NS128488;R35GM128761

Available on Infoscience
January 28, 2025
Use this identifier to reference this record
https://infoscience.epfl.ch/handle/20.500.14299/245751
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