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The whereabouts of transmembrane proteins from rat brain synaptosomes during two-dimensional gel electrophoresis
Authors:Eravci Murat  Fuxius Sandra  Broedel Oliver  Weist Stephanie  Krause Eberhard  Stephanowitz Heike  Schluter Hartmut  Eravci Selda  Baumgartner Andreas
Institution:1. Department of Radiology and Nuclear Medicine (Radiochemistry), Charité Universit?tsmedizin, Campus Benjamin Franklin, Berlin, Germany;2. A+M Proteome Science, Berlin, Germany;3. Leibniz Institute for Molecular Pharmacology (FMP), Berlin, Germany;4. Department of Internal Medicine IV ‐ Nephrology, Charité Universit?tsmedizin, Campus Benjamin Franklin, Berlin, Germany
Abstract:Little is known about what happens to transmembrane proteins (TMP) in 2-DE. In order to obtain more insight into the whereabouts of these proteins we prepared membrane-enriched synaptosomes from rat frontal cortex and washed them with 7 M urea or Na(2)CO(3). From each preparation, 200 microg protein was loaded on 2-DE gels covering the 4-7 and 6-11 pH ranges, respectively. MALDI-MS/MS analysis detected only 3 TMP among 421 identified spots. However, when the samples had been washed with Na(2)CO(3), only few well-focused spots remained detectable on the gel covering the pH 6-11 range. Instead, a heavily ruthenium-stained smear became visible at the upper edge of the gel at the location where the samples had been applied by cup loading. LC-MS/MS analysis revealed that this smear contained 38 unfocused TMP with up to 12 transmembrane helices. After transfer to the second dimension, no major areas of protein staining were left on the IPG strips. This indicates that after extraction and denaturation the TMP may form high-molecular aggregates, due to their "hydrophobic interactions". These aggregates enter the IPG strips, but do not focus regularly. They are then transferred onto the 2-DE-gels, where they remain caught at the upper edge.
Keywords:Carbonate washing  Rat brain  Synaptosomes  Transmembrane proteins  Two‐dimensional gel electrophoresis
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