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Profiling of Protease Cleavage Sites by Proteome-Derived Peptide Libraries and Quantitative Proteomics

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Protein Terminal Profiling

Part of the book series: Methods in Molecular Biology ((MIMB,volume 1574))

Abstract

Biochemical profiling of active site specificity is a crucial step to characterize proteases, which play key roles in health and disease. Here, we present a protocol using proteome-derived peptide libraries in combination with quantitative proteomics to simultaneously identify cleavage motifs N- and C-terminal to the scissile peptide bond. First, bacterial or eukaryotic cell lysate is used to generate peptide libraries. Without further chemical modification, peptide libraries are then split into control and treated (incubate with active protease) aliquots. Control and treated libraries are stable isotope-labeled, mixed, and analyzed by liquid chromatography-tandem mass spectrometry. Enriched, semi-specific peptides represent the cleavage products of the test protease and the entire peptide sequence that encompasses the scissile peptide bond is reconstructed bioinformatically. The method is fast, cost-effective, and suited for proteases with narrow or loose specificity.

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Correspondence to Oliver Schilling .

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Chen, Cy., Mayer, B., Schilling, O. (2017). Profiling of Protease Cleavage Sites by Proteome-Derived Peptide Libraries and Quantitative Proteomics. In: Schilling, O. (eds) Protein Terminal Profiling. Methods in Molecular Biology, vol 1574. Humana Press, New York, NY. https://doi.org/10.1007/978-1-4939-6850-3_14

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  • DOI: https://doi.org/10.1007/978-1-4939-6850-3_14

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  • Publisher Name: Humana Press, New York, NY

  • Print ISBN: 978-1-4939-6849-7

  • Online ISBN: 978-1-4939-6850-3

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