Literature DB >> 22258423

Whole-object fluorescence lifetime setup for efficient non-imaging quantitative intracellular fluorophore measurements.

Yaniv Namer1, Lior Turgeman, Mordechai Deutsch, Dror Fixler.   

Abstract

In the present study we introduce a Whole-Object Fluorescence Life Time (wo-FLT) measurement approach for ease and a relatively inexpensive method of tracing alterations in intracellular fluorophore distribution and in the physical-chemical features of the microenvironments hosting the fluorophore. Two common fluorophores, Rhodamine 123 and Acridine Orange, were used to stain U937 cells which were incubated, with and without either Carbonyl cyanide 3-chlorphenylhydrazon or the apoptosis inducer H(2)O(2). The wo-FLT, which is a non-imaging quantitative measurement, was able to detect several fluorescence decay components and corresponding weights in a single cell resolution. Following cell treatment, both decay time and weight were altered. Results suggest that the prominent factor responsible for these alterations and in some cases to a shift in emission spectrum as well, is the intracellular fluorophore local concentration. In this study it was demonstrated that the proposed wo-FLT method is superior to color fluorescence based imaging in cases where the emission spectrum of a fluorophore remains unchanged during the investigated process. The proposed wo-FLT approach may be of particular importance when direct imaging is impossible.

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Year:  2012        PMID: 22258423     DOI: 10.1007/s10895-011-1025-x

Source DB:  PubMed          Journal:  J Fluoresc        ISSN: 1053-0509            Impact factor:   2.217


  24 in total

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Authors:  A Squire; P J Verveer; P I Bastiaens
Journal:  J Microsc       Date:  2000-02       Impact factor: 1.758

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3.  Implication toward a simple strategy to generate efficiency-tunable fluorescence resonance energy transfer emission: intertwining medium-polarity-sensitive intramolecular charge transfer emission to fluorescence resonance energy transfer.

Authors:  Bijan Kumar Paul; Anuva Samanta; Nikhil Guchhait
Journal:  J Phys Chem A       Date:  2010-05-27       Impact factor: 2.781

4.  Analysis of early apoptotic events in individual cells by fluorescence intensity and polarization measurements.

Authors:  N Zurgil; Y Shafran; D Fixler; M Deutsch
Journal:  Biochem Biophys Res Commun       Date:  2002-02-08       Impact factor: 3.575

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Journal:  Biophysik       Date:  1967

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Authors:  A V Zelenin
Journal:  Nature       Date:  1966-10-22       Impact factor: 49.962

7.  Characterization of the steady-state and dynamic fluorescence properties of the potential-sensitive dye bis-(1,3-dibutylbarbituric acid)trimethine oxonol (Dibac4(3)) in model systems and cells.

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Journal:  Chem Phys Lipids       Date:  1994-02       Impact factor: 3.329

8.  Caspase-dependent and -independent events in apoptosis induced by hydrogen peroxide.

Authors:  D K Kim; E S Cho; H D Um
Journal:  Exp Cell Res       Date:  2000-05-25       Impact factor: 3.905

9.  Mitochondrial and plasma membrane potentials cause unusual accumulation and retention of rhodamine 123 by human breast adenocarcinoma-derived MCF-7 cells.

Authors:  S Davis; M J Weiss; J R Wong; T J Lampidis; L B Chen
Journal:  J Biol Chem       Date:  1985-11-05       Impact factor: 5.157

10.  Dynamic compression modulates chondrocyte proliferation and matrix biosynthesis in chitosan/gelatin scaffolds.

Authors:  Peng-Yuan Wang; Hsiang-Hong Chow; Juin-Yih Lai; Hsuan-Liang Liu; Wei-Bor Tsai
Journal:  J Biomed Mater Res B Appl Biomater       Date:  2009-10       Impact factor: 3.368

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