Xi Deng scite author profile

Xi Deng

3Publications

18Citation Statements Received

45Citation Statements Given

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162

Affiliations

Technische Universität Braunschweig

Publications

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The challenge to quantify proteins with charge trains due to isoforms or conformers

et al. 2011

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Single proteins separated by 2-DE often show multiple spots spreading along the first dimension. In many cases, such charge trains are explained by isoform differences or by putative post-translational modifications including phosphorylation, glycosylation and others. We now report that individual spots of such charge trains on 2-D gels in fact often represent the same protein, but, apparently due to conformational changes, segregate to different isoelectric points. If MS analysis reveals protein identity, we therefore suggest integrating all individual spots within a charge train for quantification. Especially in quality control of pharmaceutical proteins, the integration of the spot groups of all active contents is preferable in order to obtain reproducible and reasonable quantitative results. However, most commercial software packages for gel analysis integrate the signals spot-wise. We provide an improved quantification tool for proteins with charge train groups. This calculation can be implemented using the MATLAB software and the self-developed "Correct Integration Software System" or the commercial software package Delta2D.

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Improving precision in gel electrophoresis by stepwisely decreasing variance components

Schröder

Brandmüller

Deng

et al. 2009

Journal of Pharmaceutical and Biomedical Analysis

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Quantitative gel electrophoresis: New records in precision by elaborated staining and detection protocols

et al. 2011

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Gel electrophoresis (GE) is a very common analytical technique for proteome research and protein analysis. Despite being developed decades ago, there is still a considerable need to improve its precision. Using the fluorescence of Colloidal Coomassie Blue -stained proteins in near-infrared (NIR), the major error source caused by the unpredictable background staining is strongly reduced. This result was generalized for various types of detectors. Since GE is a multi-step procedure, standardization of every single step is required. After detailed analysis of all steps, the staining and destaining were identified as the major source of the remaining variation. By employing standardized protocols, pooled percent relative standard deviations of 1.2-3.1% for band intensities were achieved for one-dimensional separations in repetitive experiments. The analysis of variance suggests that the same batch of staining solution should be used for gels of one experimental series to minimize day-to-day variation and to obtain high precision.

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Xi Deng

The challenge to quantify proteins with charge trains due to isoforms or conformers

Improving precision in gel electrophoresis by stepwisely decreasing variance components

Quantitative gel electrophoresis: New records in precision by elaborated staining and detection protocols

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