TY - JOUR
T1 - Optimization of paper bridge loading for 2-DE analysis in the basic pH region
T2 - Application to the mitochondrial subproteome
AU - Kane, Lesley A.
AU - Yung, Christina K.
AU - Agnetti, Giulio
AU - Neverova, Irina
AU - Van Eyk, Jennifer E.
PY - 2006/11
Y1 - 2006/11
N2 - Separation of basic proteins with 2-DE presents technical challenges involving protein precipitation, load limitations, and streaking. Cardiac mitochondria are enriched in basic proteins and difficult to resolve by 2-DE. We investigated two methods, cup and paper bridge, for sample loading of this subproteome into the basic range (pH 6-11) gels. Paper bridge loading consistently produced improved resolution of both analytical and preparative protein loads. A unique benefit of this technique is that proteins retained in the paper bridge after loading basic gels can be reloaded onto lower pH gradients (pH 4-7), allowing valued samples to be analyzed on multiple pH ranges.
AB - Separation of basic proteins with 2-DE presents technical challenges involving protein precipitation, load limitations, and streaking. Cardiac mitochondria are enriched in basic proteins and difficult to resolve by 2-DE. We investigated two methods, cup and paper bridge, for sample loading of this subproteome into the basic range (pH 6-11) gels. Paper bridge loading consistently produced improved resolution of both analytical and preparative protein loads. A unique benefit of this technique is that proteins retained in the paper bridge after loading basic gels can be reloaded onto lower pH gradients (pH 4-7), allowing valued samples to be analyzed on multiple pH ranges.
KW - Mitochondria
KW - Paper bridge loading
KW - Two-dimensional gel electrophoresis
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U2 - 10.1002/pmic.200600267
DO - 10.1002/pmic.200600267
M3 - Article
C2 - 17022103
AN - SCOPUS:33751082637
SN - 1615-9853
VL - 6
SP - 5683
EP - 5687
JO - Proteomics
JF - Proteomics
IS - 21
ER -