Literature DB >> 18001079

The effects of shared peptides on protein quantitation in label-free proteomics by LC/MS/MS.

Shuangshuang Jin1, Donald S Daly, David L Springer, John H Miller.   

Abstract

Assessment of differential protein abundance from the observed properties of detected peptides is an essential part of protein profiling based on shotgun proteomics. However, the abundance observed for shared peptides may be due to contributions from multiple proteins that are affected differently by a given treatment. Excluding shared peptides eliminates this ambiguity but may significantly decrease the number of proteins for which abundance estimates can be obtained. Peptide sharing within a family of biologically related proteins does not cause ambiguity if family members have a common response to treatment. On the basis of this concept, we have developed an approach for including shared peptides in the analysis of differential protein abundance in protein profiling. Data from a recent proteomics study of lung tissue from mice exposed to lipopolysaccharide, cigarette smoke, and a combination of these agents are used to illustrate our method. Starting from data where about half of the implicated database protein involved shared peptides, 82% of the affected proteins were grouped into families, based on FASTA annotation, with closure on peptide sharing. In many cases, a common abundance relative to control was sufficient to explain ion-current peak areas for peptides, both unique and shared, that identified biologically related proteins in a peptide-sharing closure group. On the basis of these results, we propose that peptide-sharing closure groups provide a way to include abundance data for shared peptides in quantitative protein profiling by high-throughput mass spectrometry.

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Year:  2007        PMID: 18001079     DOI: 10.1021/pr0704175

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


  15 in total

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10.  Platelet proteome changes associated with diabetes and during platelet storage for transfusion.

Authors:  David L Springer; John H Miller; Sherry L Spinelli; Ljiljana Pasa-Tolic; Samuel O Purvine; Donald S Daly; Richard C Zangar; Shuangshuang Jin; Neil Blumberg; Charles W Francis; Mark B Taubman; Ann E Casey; Steven D Wittlin; Richard P Phipps
Journal:  J Proteome Res       Date:  2009-05       Impact factor: 4.466

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