Apoptosis
Global Sequencing of Proteolytic Cleavage Sites in Apoptosis by Specific Labeling of Protein N Termini
08/09/2008
The nearly 600
proteases in the human genome regulate a diversity of
biological processes, including programmed cell
death. Comprehensive characterization of protease
signaling in complex biological samples is limited by
available proteomic methods. We have developed a
general approach for global identification of
proteolytic cleavage sites using an engineered enzyme
to selectively biotinylate free protein N termini for
positive enrichment of corresponding N-terminal
peptides. Using this method to study apoptosis, we
have sequenced 333 caspase-like cleavage sites
distributed among 292 protein substrates. These sites
are generally not predicted by in vitro caspase
substrate specificity but can be used to predict
other physiological caspase cleavage sites.
Structural bioinformatic studies show that caspase
cleavage sites often appear in surface-accessible
loops and even occasionally in helical regions.
Strikingly, we also find that a disproportionate
number of caspase substrates physically interact,
suggesting that these dimeric proteases target
protein complexes and networks to elicit apoptosis.
Cell, Volume 134, Issue 5, 5 September 2008, Pages 866-876
Cell, Volume 134, Issue 5, 5 September 2008, Pages 866-876
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