Literature DB >> 22527512

Combining ultracentrifugation and peptide termini group-specific immunoprecipitation for multiplex plasma protein analysis.

Sonja Volk1, Thomas D Schreiber, David Eisen, Calvin Wiese, Hannes Planatscher, Christopher J Pynn, Dieter Stoll, Markus F Templin, Thomas O Joos, Oliver Pötz.   

Abstract

Blood plasma is a valuable source of potential biomarkers. However, its complexity and the huge dynamic concentration range of its constituents complicate its analysis. To tackle this problem, an immunoprecipitation strategy was employed using antibodies directed against short terminal epitope tags (triple X proteomics antibodies), which allow the enrichment of groups of signature peptides derived from trypsin-digested plasma. Isolated signature peptides are subsequently detected using MALDI-TOF/TOF mass spectrometry. Sensitivity of the immunoaffinity approach was, however, compromised by the presence of contaminant peaks derived from the peptides of nontargeted high abundant proteins. A closer analysis of the enrichment strategy revealed nonspecific peptide binding to the solid phase affinity matrix as the major source of the contaminating peptides. We therefore implemented a sucrose density gradient ultracentrifugation separation step into the procedure. This yielded a 99% depletion of contaminating peptides from a sucrose fraction containing 70% of the peptide-antibody complexes and enabled the detection of the previously undetected low abundance protein filamin-A. Assessment of this novel approach using 15 different triple X proteomics antibodies demonstrated a more consistent detection of a greater number of targeted peptides and a significant reduction in the intensity of nonspecific peptides. Ultracentrifugation coupled with immunoaffinity MS approaches presents a powerful tool for multiplexed plasma protein analysis without the requirement for demanding liquid chromatography separation techniques.

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Year:  2012        PMID: 22527512      PMCID: PMC3394961          DOI: 10.1074/mcp.O111.015438

Source DB:  PubMed          Journal:  Mol Cell Proteomics        ISSN: 1535-9476            Impact factor:   5.911


  48 in total

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

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

Authors:  Tao Liu; Wei-Jun Qian; Heather M Mottaz; Marina A Gritsenko; Angela D Norbeck; Ronald J Moore; Samuel O Purvine; David G Camp; Richard D Smith
Journal:  Mol Cell Proteomics       Date:  2006-07-19       Impact factor: 5.911

4.  Limitation of immunoaffinity column for the removal of abundant proteins from plasma in quantitative plasma proteomics.

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Review 5.  Strategy for surveying the proteome using affinity proteomics and mass spectrometry.

Authors:  Christer Wingren; Peter James; Carl A K Borrebaeck
Journal:  Proteomics       Date:  2009-03       Impact factor: 3.984

Review 6.  Proteome wide screening using peptide affinity capture.

Authors:  Oliver Poetz; Sibylle Hoeppe; Markus F Templin; Dieter Stoll; Thomas O Joos
Journal:  Proteomics       Date:  2009-03       Impact factor: 3.984

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8.  Efficient and specific removal of albumin from human serum samples.

Authors:  Laura F Steel; Michael G Trotter; Pamela B Nakajima; Taj S Mattu; Gregory Gonye; Timothy Block
Journal:  Mol Cell Proteomics       Date:  2003-05-16       Impact factor: 5.911

9.  High sensitivity detection of plasma proteins by multiple reaction monitoring of N-glycosites.

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Journal:  Mol Cell Proteomics       Date:  2007-07-20       Impact factor: 5.911

10.  A list of candidate cancer biomarkers for targeted proteomics.

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