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Abstract
A family of cysteine proteases, the caspases, plays a central role in the initiation
and execution phases of apoptosis. Upon activation, these enzymes cleave specific
substrates and thereby mediate many of the typical biochemical and morphological changes
in apoptotic cells, such as cell shrinkage, chromatin condensation, DNA fragmentation
and plasma membrane blebbing. Hence, the detection of activated caspases can be used
as a biochemical marker for apoptosis. Here we review a set of methods available for
characterizing and quantifying the activation of caspases, including immunoblotting,
cleavage of synthetic substrates, affinity labeling and confocal microscopy. Each
method is described in general terms and the advantages and disadvantages of each
technique are discussed.