Fluorescence lifetime imaging of fluorescent proteins as an effective quantitative tool for noninvasive study of intracellular processes

Svitlana M. Levchenko; Artem Pliss; Junle Qu

doi:10.1142/s1793545817300099

Journals >Journal of Innovative Optical Health Sciences >Volume 11 >Issue 1 >Page 1730009 > Article

Journal of Innovative Optical Health Sciences
Vol. 11, Issue 1, 1730009 (2018)

Fluorescence lifetime imaging of fluorescent proteins as an effective quantitative tool for noninvasive study of intracellular processes

Svitlana M. Levchenko¹, Artem Pliss², and Junle Qu^1、*

Author Affiliations

¹Key Laboratory of Optoelectronic Devices and Systems of Guangdong Province College of Optoelectronic Engineering, Shenzhen University Shenzhen, Guangdong Province 518060, P. R. China

²Institute for Lasers, Photonics and Biophotonics University at Buffalo, State University of New York Buffalo, NY 14260-3000, USA

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DOI: 10.1142/s1793545817300099 Cite this Article

Svitlana M. Levchenko, Artem Pliss, Junle Qu. Fluorescence lifetime imaging of fluorescent proteins as an effective quantitative tool for noninvasive study of intracellular processes[J]. Journal of Innovative Optical Health Sciences, 2018, 11(1): 1730009 Copy Citation Text

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Abstract

Fluorescence lifetime imaging (FLIM) is an effective noninvasive bioanalytical tool based on measuring fluorescent lifetime of fluorophores. A growing number of FLIM studies utilizes genetically engineered fluorescent proteins targeted to specific subcellular structures to probe local molecular environment, which opens new directions in cell science. This paper highlights the unconventional applications of FLIM for studies of molecular processes in diverse organelles of live cultured cells.

Keywords

bioimaging Fluorescence lifetime imaging fluorescent proteins intracellular processes

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