Use of Fluorescently Labeled Caspase Inhibitors as Affinity Labels to Detect Activated Caspases

Activation of caspases is the key event of apoptosis and different approaches were developed to assay it To detect their activation in situ, we applied fluorochrome labeled inhibitors of caspases (FLICA) as affinity labels of active centers of these enzymes. The FLICA ligands are fluorescein or sulf...

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Bibliographic Details
Published in:Human cell : official journal of Human Cell Research Society 2002-02, Vol.15 (1), p.1-12
Main Authors: Grabarek, Jerzy, Amstad, Paul, Darzynkiewicz, Zbigniew
Format: Article
Language:English
Subjects:
Affinity Labels
Apoptosis
apoptotic index
Caspase Inhibitors
Caspases - analysis
Cells, Cultured
enzyme active center
Enzyme Inhibitors
FLICA
Flow Cytometry
Fluoresceins
Fluorescent Dyes
Humans
laser scanning cytometry (LSC)
Microscopy, Fluorescence
stathmo‐apoptosis
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Summary:Activation of caspases is the key event of apoptosis and different approaches were developed to assay it To detect their activation in situ, we applied fluorochrome labeled inhibitors of caspases (FLICA) as affinity labels of active centers of these enzymes. The FLICA ligands are fluorescein or sulforhodamine conjugated peptide‐fluoromethyl ketones diat covalently bind to enzymatic centers of caspases with 1:1 stoichiometry. The specificity of FLICA towards individual caspases is provided by the peptide sequence of amino acids. Exposure of live cells to FLICA results in uptake of these ligands and their binding to activated caspases; unbound FLICA is removed by cell rinse. Cells labeled with FLICA can be examined by fluorescence microscopy or subjected to quantitative analysis by cytometry. Intracellular binding sites of FLICA are consistent with known localization of caspases. Covalent binding of FLICA allowed us to identify the labeled proteins by immunoblotting: the proteins that bound individual FLICAs had molecular weight between 17 and 22 kDa, which corresponds to large subunits of the caspases. Detection of caspases activation by FLICA can be combined with other markers of apoptosis or cell cycle for multiparametric analysis. Because FLICA are caspase inhibitors they arrest the process of apoptosis preventing cell disintegration. The stathmo‐apoptotic method was developed, therefore, that allows one to assay cumulative apoptotic index over long period of time and estimate the rate of cell entry into apoptosis for large cell populations. FLICA offers a rapid and convenient assay of caspases activation and can also be used to accurately estimate the incidence of apoptosis.
ISSN:0914-7470
1749-0774
DOI:10.1111/j.1749-0774.2002.tb00094.x