Literature DB >> 17547438

Identification of proteolytic cleavage sites by quantitative proteomics.

Mari Enoksson1, Jingwei Li, Melanie M Ivancic, John C Timmer, Eric Wildfang, Alexey Eroshkin, Guy S Salvesen, W Andy Tao.   

Abstract

The identification of natural substrates and their cleavage sites is pivotal to defining proteolytic pathways. Here we report a novel strategy for the identification of the signature of proteolytic cleavage events based on quantitative proteomics. Lysine residues in proteins are blocked by guanidination so that free N-terminals can be labeled with amine-specific iTRAQ reagents. The quantitative nature of iTRAQ reagents allows us to distinguish N-terminals newly formed by proteolytic treatment (neoepitopes) from original N-terminals in proteins. Proteins are digested with trypsin and analyzed using MALDI-TOF/TOF mass spectrometry. Peptides labeled with iTRAQ reagents are distinguished from other peptides by exhibiting intense signature ions in tandem mass spectrometry analysis. A corresponding data acquisition strategy was developed to specifically analyze iTRAQ tagged N-terminal peptides. To validate the procedure, we examined a set of recombinant Escherichia coli proteins that have predicted caspase-3 cleavage motifs. The protein mixture was treated with active or inactive caspase-3 and subsequently labeled with two different iTRAQ reagents. Mass spectrometric analysis located 10 cleavage sites, all corresponding to caspase-3 consensus. Spiking caspase-cleaved substrate into a human cell lysate demonstrated the high sensitivity of the procedure. Moreover, we were able to identify proteolytic cleavage products associated with the induction of cell-free apoptosis. Together, these data reveal a novel application for iTRAQ technology for the detection of proteolytic substrates.

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Year:  2007        PMID: 17547438     DOI: 10.1021/pr0701052

Source DB:  PubMed          Journal:  J Proteome Res        ISSN: 1535-3893            Impact factor:   4.466


  28 in total

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5.  Selecting protein N-terminal peptides by combined fractional diagonal chromatography.

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6.  Analyzing protease specificity and detecting in vivo proteolytic events using tandem mass spectrometry.

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Review 7.  New approaches for dissecting protease functions to improve probe development and drug discovery.

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8.  A statistics-based platform for quantitative N-terminome analysis and identification of protease cleavage products.

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Journal:  Mol Cell Proteomics       Date:  2010-03-20       Impact factor: 5.911

9.  Structural and kinetic determinants of protease substrates.

Authors:  John C Timmer; Wenhong Zhu; Cristina Pop; Tim Regan; Scott J Snipas; Alexey M Eroshkin; Stefan J Riedl; Guy S Salvesen
Journal:  Nat Struct Mol Biol       Date:  2009-09-20       Impact factor: 15.369

10.  Tags for labeling protein N-termini with subtiligase for proteomics.

Authors:  Hikari A I Yoshihara; Sami Mahrus; James A Wells
Journal:  Bioorg Med Chem Lett       Date:  2008-08-19       Impact factor: 2.823

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