Literature DB >> 16229651

Tracing apoptosis and stimulation in individual cells by fluorescence intensity and anisotropy decay.

Dror Fixler1, Reuven Tirosh, Naomi Zurgil, Mordechai Deutsch.   

Abstract

Presented is the use of fluorescence lifetime (FLT), anisotropy decay, and associated parameters as differential indicators of cellular activity. A specially designed combination of a frequency mode based time resolved microscope and a picoliter well-per-cell array have been used to perform temporal measurements in individual cells under various biological conditions. Two biological models have been examined: mitogenic activation of peripheral blood mononuclear cells (PBMC) and induction of programmed cell death (apoptosis) in Jurkat T cells (JTC). The FLT of fluorescein stained PBMC was found to increase from 4+/-0.02 to 4.5+/-0.025 ns due to mitogenic activation, whereas during apoptosis in fluorescein stained JTC, the FLT remained constant. Notably, the rotational correlation times changed in both models: decreased in PBMC from 2.5+/-0.08 to 2+/-0.1 ns, and increased in JTC from 2.1+/-0.07 to 3.3+/-0.09 ns. FLT and rotational correlation time were used to calculate the steady state fluorescence anisotropy (FA) which was compared to directly measured FA values. The present study suggests that in addition to bioindication, the said parameters can provide valuable information about cellular mechanisms that may involve complex molecular diffusion dynamics, as well as information about structural changes that a cellular fluorophore undergoes in the course of cell activation. 2005 Society of Photo-Optical Instrumentation Engineers.

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Year:  2005        PMID: 16229651     DOI: 10.1117/1.1924712

Source DB:  PubMed          Journal:  J Biomed Opt        ISSN: 1083-3668            Impact factor:   3.170


  7 in total

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

Authors:  Yaniv Namer; Lior Turgeman; Mordechai Deutsch; Dror Fixler
Journal:  J Fluoresc       Date:  2012-01-20       Impact factor: 2.217

2.  Molecular fluorescence, phosphorescence, and chemiluminescence spectrometry.

Authors:  Kristin A Fletcher; Sayo O Fakayode; Mark Lowry; Sheryl A Tucker; Sharon L Neal; Irene W Kimaru; Matthew E McCarroll; Gabor Patonay; Philip B Oldham; Oleksandr Rusin; Robert M Strongin; Isiah M Warner
Journal:  Anal Chem       Date:  2006-06-15       Impact factor: 6.986

3.  Fluorophore spectroscopy in aqueous glycerol solution: the interactions of glycerol with the fluorophore.

Authors:  Haim Feldman; Mark A Iron; Dror Fixler; Sergei Moshkov; Naomi Zurgil; Elena Afrimzon; Mordechai Deutsch
Journal:  Photochem Photobiol Sci       Date:  2021-10-05       Impact factor: 3.982

4.  Diffusion Reflection and Fluorescence Lifetime Imaging Microscopy Study of Fluorophore-Conjugated Gold Nanoparticles or Nanorods in Solid Phantoms.

Authors:  Dror Fixler; Tsviya Nayhoz; Krishanu Ray
Journal:  ACS Photonics       Date:  2014-08-25       Impact factor: 7.529

5.  Fluorescence Lifetime Imaging Microscopy, a Novel Diagnostic Tool for Metastatic Cell Detection in the Cerebrospinal Fluid of Children with Medulloblastoma.

Authors:  Sivan Gershanov; Shalom Michowiz; Helen Toledano; Gilad Yahav; Orit Barinfeld; Avraham Hirshberg; Haim Ben-Zvi; Gabriel Mircus; Mali Salmon-Divon; Dror Fixler; Nitza Goldenberg-Cohen
Journal:  Sci Rep       Date:  2017-06-16       Impact factor: 4.379

6.  The Scattering of Gold Nanorods Combined with Differential Uptake, Paving a New Detection Method for Macrophage Subtypes Using Flow Cytometery.

Authors:  Ruchira Chakraborty; Dorit Leshem-Lev; Ran Kornowski; Dror Fixler
Journal:  Nano Lett       Date:  2020-10-16       Impact factor: 11.189

7.  Time-averaged fluorescence intensity analysis in fluorescence fluctuation polarization sensitive experiments.

Authors:  Lior Turgeman; Dror Fixler
Journal:  Biomed Opt Express       Date:  2013-05-13       Impact factor: 3.732

  7 in total

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