Literature DB >> 15817064

AB-plot assisted determination of fluorophore mixtures in a fluorescence lifetime microscope using spectra or quenchers.

Q S Hanley1, A H A Clayton.   

Abstract

Most treatments of frequency domain lifetime measurements indicate that a set of measurements must be made at multiple frequencies in order to determine the lifetimes of the components in a mixture. Although this is the case in general, under special conditions, single-frequency data can resolve multiple lifetimes. Here, data are presented showing several approaches to determining fluorescence lifetimes in two-component mixtures using single-frequency data. Common to all of the procedures presented is exploitation of variations in the relative contributions of a particular fluorophore to the total fluorescence from a mixture of fluorophores. This variation can be produced intentionally by observing a number of samples which contain different relative amounts of the fluorophores. It can be produced fortuitously by observing spatial variations in a mixture of fluorophores in a specimen or set of specimens observed with a lifetime imaging system. It can also be produced by examination of the lifetime spectrum obtained from a fluorophore mixture or by varying the concentration of a quencher in a fluorophore mixture, in which the two fluorophores have different rate constants for quenching. In many instances, the set of approaches presented here will be unsuitable for examination of arbitrary samples of unknown composition for which the multifrequency approach should be used. However, measurements produced using single-frequency methods may be applied to good effect for controlled experiments having defined fluorophores or sets of fluorophores, particularly in the case of biological lifetime imaging studies.

Year:  2005        PMID: 15817064     DOI: 10.1111/j.1365-2818.2005.01463.x

Source DB:  PubMed          Journal:  J Microsc        ISSN: 0022-2720            Impact factor:   1.758


  10 in total

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2.  Applications of phasors to in vitro time-resolved fluorescence measurements.

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3.  Quantitative lifetime unmixing of multiexponentially decaying fluorophores using single-frequency fluorescence lifetime imaging microscopy.

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Journal:  Biophys J       Date:  2008-03-21       Impact factor: 4.033

4.  Quantitative analysis of fluorescence lifetime imaging made easy.

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5.  Investigating protein-protein interactions in living cells using fluorescence lifetime imaging microscopy.

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Journal:  Nat Protoc       Date:  2011-08-11       Impact factor: 13.491

6.  Red-shifted fluorescent proteins monitor enzymatic activity in live HT-1080 cells with fluorescence lifetime imaging microscopy (FLIM).

Authors:  J P Eichorst; R M Clegg; Y Wang
Journal:  J Microsc       Date:  2012-10       Impact factor: 1.758

7.  Processing of fluorescence lifetime image using modified phasor approach: homo-FRET from the acceptor.

Authors:  Yanzhou Zhou; Yulei Bai; Ci Chen; John M Dickenson
Journal:  J Fluoresc       Date:  2013-03-15       Impact factor: 2.217

8.  Advanced Fluorescence Microscopy Methods to Study Dynamics of Fluorescent Proteins In Vivo.

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Journal:  Methods Mol Biol       Date:  2023

9.  How many photons are needed for FRET imaging?

Authors:  Alessandro Esposito
Journal:  Biomed Opt Express       Date:  2020-01-30       Impact factor: 3.732

10.  Evaluation of Caspase-3 Activity During Apoptosis with Fluorescence Lifetime-Based Cytometry Measurements and Phasor Analyses.

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Journal:  Cytometry A       Date:  2020-08-25       Impact factor: 4.355

  10 in total

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