Research Article

Industrial-scale proteomics: From liters of plasma to chemically synthesized proteins

  1. Keith Rose1,*,
  2. Lydie Bougueleret1,
  3. Thierry Baussant1,
  4. Günter Böhm1,
  5. Paolo Botti1,
  6. Jacques Colinge1,
  7. Isabelle Cusin1,
  8. Hubert Gaertner1,
  9. Anne Gleizes1,
  10. Manfred Heller1,
  11. Silvia Jimenez1,
  12. Andrew Johnson1,
  13. Martin Kussmann1,
  14. Laure Menin1,
  15. Christoph Menzel1,
  16. Frederic Ranno1,
  17. Patricia Rodriguez-Tomé1,
  18. John Rogers1,
  19. Cedric Saudrais1,
  20. Matteo Villain1,
  21. Diana Wetmore1,
  22. Amos Bairoch1,2,
  23. Denis Hochstrasser1,3

Article first published online: 22 APR 2004

DOI: 10.1002/pmic.200300718

Issue

PROTEOMICS

PROTEOMICS

Special Issue: Proceedings of the AEPS Meeting, Melbourne, Australia 27-28 September 2003

Volume 4, Issue 7, pages 2125–2150, July 2004

Additional Information

How to Cite

Rose, K., Bougueleret, L., Baussant, T., Böhm, G., Botti, P., Colinge, J., Cusin, I., Gaertner, H., Gleizes, A., Heller, M., Jimenez, S., Johnson, A., Kussmann, M., Menin, L., Menzel, C., Ranno, F., Rodriguez-Tomé, P., Rogers, J., Saudrais, C., Villain, M., Wetmore, D., Bairoch, A. and Hochstrasser, D. (2004), Industrial-scale proteomics: From liters of plasma to chemically synthesized proteins. PROTEOMICS, 4: 2125–2150. doi: 10.1002/pmic.200300718

Author Information

  1. 1

    GeneProt, Geneva, Switzerland

  2. 2

    Swiss Institute of Bioinformatics, CMU, Geneva, Switzerland

  3. 3

    University Hospital of Geneva, Geneva, Switzerland

*Ph.D., GeneProt, 2 rue Pré-de-la-Fontaine, CP125, CH-1217 Meyrin 2, Switzerland Fax: +41-22-719-39-70

Publication History

  1. Issue published online: 22 JUN 2004
  2. Article first published online: 22 APR 2004
  3. Manuscript Received: 11 NOV 2003

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Keywords:

  • Industrial-scale;
  • Mass spectrometry;
  • Plasma

Abstract

Human blood plasma is a useful source of proteins associated with both health and disease. Analysis of human blood plasma is a challenge due to the large number of peptides and proteins present and the very wide range of concentrations. In order to identify as many proteins as possible for subsequent comparative studies, we developed an industrial-scale (2.5 liter) approach involving sample pooling for the analysis of smaller proteins (Mr generally < ca. 40 000 and some fragments of very large proteins). Plasma from healthy males was depleted of abundant proteins (albumin and IgG), then smaller proteins and polypeptides were separated into 12 960 fractions by chromatographic techniques. Analysis of proteins and polypeptides was performed by mass spectrometry prior to and after enzymatic digestion. Thousands of peptide identifications were made, permitting the identification of 502 different proteins and polypeptides from a single pool, 405 of which are listed here. The numbers refer to chromatographically separable polypeptide entities present prior to digestion. Combining results from studies with other plasma pools we have identified over 700 different proteins and polypeptides in plasma. Relatively low abundance proteins such as leptin and ghrelin and peptides such as bradykinin, all invisible to two-dimensional gel technology, were clearly identified. Proteins of interest were synthesized by chemical methods for bioassays. We believe that this is the first time that the small proteins in human blood plasma have been separated and analyzed so extensively.

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