Improved proteome analysis of Saccharomyces cerevisiae mitochondria by free-flow electrophoresis.

Zischka, H; Weber, G; Weber, PJ; Posch, A; Braun, RJ; Bühringer, D; Schneider, U; Nissum, M; Meitinger, T; Ueffing, M; Eckerskorn, C

doi:10.1002/pmic.200300376

2003

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Titel:: Improved proteome analysis of Saccharomyces cerevisiae mitochondria by free-flow electrophoresis.
Dokumenttyp:: Journal Article; Article
Autor(en):: Zischka, H; Weber, G; Weber, PJ; Posch, A; Braun, RJ; Bühringer, D; Schneider, U; Nissum, M; Meitinger, T; Ueffing, M; Eckerskorn, C
Abstract:: The analysis of complex cellular proteomes by means of two-dimensional gel electrophoresis (2-DE) is significantly limited by the power of resolution of this technique. Although subcellular fractionation can be a fundamental first step to increase resolution, it frequently leads to preparations contaminated with other cellular structures. Here, we chose mitochondria of Saccharomyces cerevisiae to demonstrate that an integrated zone-electrophoretic purification step (ZE), with a free-flow electrophoresis device (FFE), can assist in overcoming this problem, while significantly improving their degree of purity. Whereas mitochondrial preparations isolated by means of differential centrifugation include a considerable degree of non-mitochondrial proteins (16%), this contamination could be effectually removed by the inclusion of a ZE-FFE purification step (2%). This higher degree of purity led to the identification of many more proteins from ZE-FFE purified mitochondrial protein extracts (n = 129), compared to mitochondrial protein extracts isolated by differential centrifugation (n = 80). Moreover, a marked decrease of degraded proteins was found in the ZE-FFE purified mitochondrial protein extracts. It is noteworthy that even at a low 2-DE resolution level, a four-fold higher number (17 versus 4) of presumably low abundance proteins could be identified in the ZE-FFE purified mitochondrial protein extracts. Therefore these results represent a feasible approach for an in-depth proteome analysis of mitochondria and possibly other organelles. «
The analysis of complex cellular proteomes by means of two-dimensional gel electrophoresis (2-DE) is significantly limited by the power of resolution of this technique. Although subcellular fractionation can be a fundamental first step to increase resolution, it frequently leads to preparations contaminated with other cellular structures. Here, we chose mitochondria of Saccharomyces cerevisiae to demonstrate that an integrated zone-electrophoretic purification step (ZE), with a free-flow electro... »
Zeitschriftentitel:: Proteomics
Jahr:: 2003
Band / Volume:: 3
Heft / Issue:: 6
Seitenangaben Beitrag:: 906-16
Sprache:: eng
Volltext / DOI:: doi:10.1002/pmic.200300376
PubMed:: http://view.ncbi.nlm.nih.gov/pubmed/12833514
Print-ISSN:: 1615-9853
TUM Einrichtung:: Institut für Humangenetik
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mediaTUM Gesamtbestand Einrichtungen Schools TUM School of Medicine and Health Departments Clinical Medicine Institut für Humangenetik (Prof. Winkelmann)2003