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Titlebook: Difference Gel Electrophoresis; Methods and Protocol Kay Ohlendieck Book 2018 Springer Science+Business Media LLC 2018 DIGE.fluorescence im

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H. A. Snellen,H. C. Hemker,J. H. Bemmelities recorded at the different wavelengths are integrated and the ratio between volumes normalized to that of the internal standard. This provides an immediate appreciation of protein amount variations under the different conditions tested. In addition, proteins of interest can still be excised and
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The Need for Quantitation in Cardiology of tissue protein compositions. Comparing tissue groups under different conditions is crucially important for advancing the biomedical field by characterization of cellular processes, understanding pathophysiological development and tissue biomarker discovery. This chapter discusses 2D-DIGE as a co
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2D-DIGE and Fluorescence Image Analysisback of classical two-dimensional gel-electrophoresis. However, once 2D-gels are obtained, they must undergo a quite articulated multistep image analysis procedure before the final differential analysis via statistical mono- and multivariate methods. Here, the main steps of image analysis software a
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Native DIGE: Efficient Tool to Elucidate Protein Interactomesructural and functional heterogeneity to the proteome. One needs to consider this aspect while studying changes in abundance or activities of proteins in response to any physiological stimulus. Abundance changes in components of a given proteome can be best visualized and quantified using electropho
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Comparative Two-Dimensional Fluorescence Gel Electrophoresist for protein spots visualized on 2D polyacrylamide gels. This is particularly important for samples, which need to be compared without the availability of replicates and thus cannot be studied using differential gel electrophoresis (DIGE). CoFGE corrects for gel-to-gel variability by co-running wit
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