High-throughput fluorescence lifetime imaging flow cytometry

Author:

Kanno HiroshiORCID,Hiramatsu KotaroORCID,Mikami HideharuORCID,Nakayashiki Atsushi,Yamashita Shota,Nagai Arata,Okabe Kohki,Li Fan,Yin Fei,Tominaga Keita,Bicer Omer Faruk,Noma Ryohei,Kiani Bahareh,Efa Olga,Büscher MartinORCID,Wazawa Tetsuichi,Sonoshita Masahiro,Shintaku Hirofumi,Nagai TakeharuORCID,Braun SigurdORCID,Houston Jessica P.ORCID,Rashad Sherif,Niizuma KuniyasuORCID,Goda KeisukeORCID

Abstract

AbstractFlow cytometry is a vital tool in biomedical research and laboratory medicine. However, its accuracy is often compromised by undesired fluctuations in fluorescence intensity. While fluorescence lifetime imaging microscopy (FLIM) bypasses this challenge as fluorescence lifetime remains unaffected by such fluctuations, the full integration of FLIM into flow cytometry has yet to be demonstrated due to speed limitations. Here we overcome the speed limitations in FLIM, thereby enabling high-throughput FLIM flow cytometry at a high rate of over 10,000 cells per second. This is made possible by using dual intensity-modulated continuous-wave beam arrays with complementary modulation frequency pairs for fluorophore excitation and acquiring fluorescence lifetime images of rapidly flowing cells. Moreover, our FLIM system distinguishes subpopulations in male rat glioma and captures dynamic changes in the cell nucleus induced by an anti-cancer drug. FLIM flow cytometry significantly enhances cellular analysis capabilities, providing detailed insights into cellular functions, interactions, and environments.

Publisher

Springer Science and Business Media LLC

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