| Literature DB >> 28986795 |
Matias Pasquali1,2, Tommaso Serchi3, Sebastien Planchon3, Jenny Renaut3.
Abstract
The two-dimensional difference gel electrophoresis method is a valuable approach for proteomics. The method, using cyanine fluorescent dyes, allows the co-migration of multiple protein samples in the same gel and their simultaneous detection, thus reducing experimental and analytical time. 2D-DIGE, compared to traditional post-staining 2D-PAGE protocols (e.g., colloidal Coomassie or silver nitrate), provides faster and more reliable gel matching, limiting the impact of gel to gel variation, and allows also a good dynamic range for quantitative comparisons. By the use of internal standards, it is possible to normalize for experimental variations in spot intensities and gel patterns. Here we describe the experimental steps we follow in our routine 2D-DIGE procedure that we then apply to multiple biological questions.Entities:
Keywords: 2D-DIGE; Animals; Electrophoresis; Fungi; Isoelectrofocusing; Plants; Proteomics; SDS-PAGE
Mesh:
Year: 2017 PMID: 28986795 DOI: 10.1007/978-1-4939-7231-9_17
Source DB: PubMed Journal: Methods Mol Biol ISSN: 1064-3745