Single-Cell Biochemical Multiplexing by Multidimensional Phasor Demixing and Spectral Fluorescence Lifetime Imaging Microscopy

被引:3
|
作者
Haas, Kalina T. [1 ,2 ]
Fries, Maximilian W. [1 ]
Venkitaraman, Ashok R. [1 ]
Esposito, Alessandro [1 ]
机构
[1] Univ Cambridge, Med Res Council Canc Unit, Cambridge, England
[2] Univ Paris Saclay, Inst Jean ierre Bourgin, INRAE, AgroParisTech, Versailles, France
来源
FRONTIERS IN PHYSICS | 2021年 / 9卷 / 09期
基金
英国惠康基金; 英国医学研究理事会;
关键词
sFLIM; FRET biosensors; TCSPC; spectral demixing; biochemical multiplexing; RESONANCE ENERGY-TRANSFER; FREQUENCY-DOMAIN; SIGNALING EVENTS; FRET MICROSCOPY; PROTEIN; FLIM; BIOSENSORS; REPRESENTATION; CAMERA;
D O I
10.3389/fphy.2021.637123
中图分类号
O4 [物理学];
学科分类号
0702 ;
摘要
Revealing mechanisms underpinning cell function requires understanding the relationship between different biochemical reactions in living cells. However, our capabilities to monitor more than two biochemical reactions in living cells are limited. Therefore, the development of methods for real-time biochemical multiplexing is of fundamental importance. Here, we show that data acquired with multicolor (mcFLIM) or spectrally resolved (sFLIM) fluorescence lifetime imaging can be conveniently described with multidimensional phasor transforms. We demonstrate a computational framework capable of demixing three Forster resonance energy transfer (FRET) probes and quantifying multiplexed biochemical activities in single living cells. We provide a comparison between mcFLIM and sFLIM suggesting that sFLIM might be advantageous for the future development of heavily multiplexed assays. However, mcFLIM-more readily available with commercial systems-can be applied for the concomitant monitoring of three enzymes in living cells without significant losses.
引用
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页数:14
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