Difference gel electrophoresis

被引:75
|
作者
Minden, Jonathan S. [1 ]
Dowd, Susan R. [1 ]
Meyer, Helmut E. [2 ]
Stuehler, Kai [2 ]
机构
[1] Carnegie Mellon Univ, Dept Biol Sci, Pittsburgh, PA 15213 USA
[2] Ruhr Univ Bochum, Med Proteom Ctr, Bochum, Germany
关键词
2-D-Difference gel electrophoresis; Biomarker; Differential proteome analysis; Fluorescence dye saturation labeling; Microdissection; PROTEOMIC EXPRESSION ANALYSIS; 2-D DIGE; QUANTITATIVE PROTEOMICS; ARABIDOPSIS-THALIANA; SCHIZOSACCHAROMYCES-POMBE; HEPATOCELLULAR-CARCINOMA; LASER MICRODISSECTION; BIOMARKER DISCOVERY; SIGNAL-TRANSDUCTION; PROTEIN EXPRESSION;
D O I
10.1002/elps.200900098
中图分类号
Q5 [生物化学];
学科分类号
071010 ; 081704 ;
摘要
Difference gel electrophoresis 9DIGE) was invented to circumvent the inherent variability of 2-DE. This variability is a natural consequence of separating thousands of proteins over a large space, such as a 15 x 20 cm slab of polyacrylamide gel. The originators of 2-DE envisioned being able to compare cancerous cells and normal cells to understand what makes these cells different. Gel-to-gel variability made this an extremely difficult task. We reasoned that if both samples could be run on the same gel, then the inherent variability would be obviated. Thus, we created matched sets of fluorescent dyes that allows one to compare two or three protein samples on a single gel. In the 12 years since the description of DIGE first appeared in Electrophoresis, this founding paper has been cited over 660 times. This review highlights some of the improvements and applications of DIGE. We hope these examples are illustrative of what has been done and where the field is headed.
引用
收藏
页码:S156 / S161
页数:6
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