Literature DB >> 20173099

Sampling the N-terminal proteome of human blood.

David Wildes1, James A Wells.   

Abstract

The proteomes of blood plasma and serum represent a potential gold mine of biological and diagnostic information, but challenges such as dynamic range of protein concentration have hampered efforts to unlock this resource. Here we present a method to label and isolate N-terminal peptides from human plasma and serum. This process dramatically reduces the complexity of the sample by eliminating internal peptides. We identify 772 unique N-terminal peptides in 222 proteins, ranging over six orders of magnitude in abundance. This approach is highly suited for studying natural proteolysis in plasma and serum. We find internal cleavages in plasma proteins created by endo- and exopeptidases, providing information about the activities of proteolytic enzymes in blood, which may be correlated with disease states. We also find signatures of signal peptide cleavage, coagulation and complement activation, and other known proteolytic processes, in addition to a large number of cleavages that have not been reported previously, including over 200 cleavages of blood proteins by aminopeptidases. Finally, we can identify substrates from specific proteases by exogenous addition of the protease combined with N-terminal isolation and quantitative mass spectrometry. In this way we identified proteins cleaved in human plasma by membrane-type serine protease 1, an enzyme linked to cancer progression. These studies demonstrate the utility of direct N-terminal labeling by subtiligase to identify and characterize endogenous and exogenous proteolysis in human plasma and serum.

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Year:  2010        PMID: 20173099      PMCID: PMC2842036          DOI: 10.1073/pnas.0914495107

Source DB:  PubMed          Journal:  Proc Natl Acad Sci U S A        ISSN: 0027-8424            Impact factor:   11.205


  41 in total

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5.  Differences among techniques for high-abundant protein depletion.

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Journal:  Proteomics       Date:  2005-08       Impact factor: 3.984

6.  Evaluation of multiprotein immunoaffinity subtraction for plasma proteomics and candidate biomarker discovery using mass spectrometry.

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Review 7.  Structure and function of C3a anaphylatoxin.

Authors:  T E Hugli
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Review 8.  Matriptase: potent proteolysis on the cell surface.

Authors:  Karin List; Thomas H Bugge; Roman Szabo
Journal:  Mol Med       Date:  2006 Jan-Mar       Impact factor: 6.354

9.  Subtiligase: a tool for semisynthesis of proteins.

Authors:  T K Chang; D Y Jackson; J P Burnier; J A Wells
Journal:  Proc Natl Acad Sci U S A       Date:  1994-12-20       Impact factor: 11.205

10.  Challenges in deriving high-confidence protein identifications from data gathered by a HUPO plasma proteome collaborative study.

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  41 in total

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Review 2.  Proteolytic post-translational modification of proteins: proteomic tools and methodology.

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5.  Quantitative Multiplex Substrate Profiling of Peptidases by Mass Spectrometry.

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6.  Depletion of plasma albumin for proteomic analysis of Bothrops jararaca snake plasma.

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7.  Molecular biomarkers in glaucoma.

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8.  The DegraBase: a database of proteolysis in healthy and apoptotic human cells.

Authors:  Emily D Crawford; Julia E Seaman; Nick Agard; Gerald W Hsu; Olivier Julien; Sami Mahrus; Huy Nguyen; Kazutaka Shimbo; Hikari A I Yoshihara; Min Zhuang; Robert J Chalkley; James A Wells
Journal:  Mol Cell Proteomics       Date:  2012-12-20       Impact factor: 5.911

9.  Conservation of caspase substrates across metazoans suggests hierarchical importance of signaling pathways over specific targets and cleavage site motifs in apoptosis.

Authors:  E D Crawford; J E Seaman; A E Barber; D C David; P C Babbitt; A L Burlingame; J A Wells
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