Abstract
Calpains are proteases that catalyze the limited cleavage of target proteins in response to Ca(2+) signaling. Because of their involvement in pathological conditions such as post-ischemic injury and Alzheimer and Parkinson disease, calpains form a class of pharmacologically significant targets for inhibition. We have determined the sequence preference for the hydrolysis of peptide substrates of the ubiquitous mu-calpain isoform by a peptide library-based approach using the proteolytic core of mu-calpain (muI-II). The approach, first described by Turk et al. (Turk, B. E., Huang, L. L., Piro, E. T., and Cantley, L. C. (2001) Nat. Biotechnol. 19, 661-667), involved the digestion of an N-terminally acetylated degenerate peptide library in conjunction with Edman sequencing to determine the specificity for residues found at primed positions. The cleavage consensus for these positions was then used to design a second, partially degenerate library, to determine specificity at unprimed positions. We have improved upon the original methodology by using a degenerate peptide dendrimer for determination of specificity at unprimed positions. By using this modified approach, the complete cleavage specificity profile for muI-II was determined for all positions flanking the cleaved peptide. A previously known preference of calpains for hydrophobic amino acids at unprimed positions was confirmed. In addition, a novel residue specificity for primed positions was revealed to highlight the importance of these sites for substrate recognition. The optimal primed site motif (MER) was shown to be capable of directing cleavage to a specific peptide bond. Accordingly, we designed a fluorescent resonance energy transfer-based substrate with optimal cleavage motifs on the primed and non-primed sides (PLFAER). The mu-calpain core shows a far greater turnover rate for our substrate than for those based on the cleavage site of alpha-spectrin or the proteolytic sequence consensus compiled from substrate alignments.
Highlights
Calpains, a family of calcium-activated intracellular proteases, are found in animals, plants, and possibly bacteria [2]
Peptide libraries used in the determination of cleavage specificity Ac refers to an acetyl group, X refers to all 20 natural amino acids minus cysteine, Z refers to norleucine, and AHA refers to aminohexanoic acid [33]
The results obtained in this study reveal that I-II possesses a general preference for hydrophobic amino acids at unprimed positions, which is consistent with previous literature
Summary
We have determined the sequence preference for the hydrolysis of peptide substrates of the ubiquitous -calpain isoform by a peptide library-based approach using the proteolytic core of -calpain (I-II). Because of the broad substrate specificity of calpains, the determination of their optimal cleavage sequence has been elusive This is reflected in the paucity of sensitive substrates and highly specific, active site-directed inhibitors. Other attempts to deduce a sequence motif from observed cleavage sites in proteins and naturally occurring peptides revealed no consistent sequence preference, other than that observed from synthetic substrates (17, 19 –22). This suggests that higher order structural features,
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