State of the art of 2D DIGE

Georgia Arentz; Florian Weiland; Martin K Oehler; Peter Hoffmann

doi:10.1002/prca.201400119

State of the art of 2D DIGE

Proteomics Clin Appl. 2015 Apr;9(3-4):277-88. doi: 10.1002/prca.201400119. Epub 2015 Feb 19.

Authors

Georgia Arentz¹, Florian Weiland, Martin K Oehler, Peter Hoffmann

Affiliation

¹ School of Molecular and Biomedical Science, Adelaide Proteomics Centre, The University of Adelaide, Adelaide, Australia.

PMID: 25400138
DOI: 10.1002/prca.201400119

Abstract

Difference gel electrophoresis enables the accurate quantification of changes in the proteome including combinations of PTMs and protein isoform expression. Here, we review recent advances in study design, image acquisition, and statistical analysis. We also compare DIGE to established and emerging mass spectrometric analysis technologies. Despite these recent advances in MS and the still unsolved limitations of 2DE to map hydrophobic, high molecular weight proteins with extreme pIs, DIGE remains the most comprehensive top-down method to study changes in abundance of intact proteins.

Keywords: 2DE; DIGE; Gel electrophoresis; MS.

Publication types

Research Support, Non-U.S. Gov't
Review

MeSH terms

Mass Spectrometry
Proteomics / methods*
Two-Dimensional Difference Gel Electrophoresis / methods*