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Fractionation and proteomic analysis of the Walterinnesia aegyptia snake venom using OFFGEL and MALDI‐TOF‐MS techniques
Authors:Tarek Mohamed Abd El Aziz  Sandrine Bourgoin‐Voillard  Stéphanie Combemale  Rémy Beroud  Mahmoud Fadl  Michel Seve  Michel De Waard
Affiliation:1. INSERM U836, Grenoble Neuroscience Institute, LabEx Ion Channels, Science and Therapeutics, France;2. University Grenoble Alpes, Grenoble, France;3. Zoology Department, Faculty of Science, Minia University, El‐Minia, Egypt;4. INSERM, IAB, PROMETHEE Proteomic Platform, Grenoble, France;5. CHU de Grenoble, IAB, Institut de Biologie et de Pathologie, PROMETHEE Proteomic Platform, Grenoble, France;6. Smartox Biotechnology, Saint‐Martin d'Hères, France
Abstract:Animal venoms are complex mixtures of more than 100 different compounds, including peptides, proteins, and nonprotein compounds such as lipids, carbohydrates, and metal ions. In addition, the existing compounds show a wide range of molecular weights and concentrations within these venoms, making separation and purification procedures quite tedious. Here, we analyzed for the first time by MS the advantages of using the OFFGEL technique in the separation of the venom components of the Egyptian Elapidae Walterinnesia aegyptia snake compared to two classical methods of separation, SEC and RP‐HPLC. We demonstrate that OFFGEL separates venom components over a larger scale of fractions, preserve respectable resolution with regard to the presence of a given compound in adjacent fractions and allows the identification of a greater number of ions by MS (102 over 134 total ions). We also conclude that applying several separating techniques (SEC and RP‐HPLC in addition to OFFGEL) provides complementary results in terms of ion detection (21 more for SEC and 22 more with RP‐HPLC). As a result, we provide a complete list of 134 ions present in the venom of W. aegyptia by using all these techniques combined.
Keywords:MS  OFFGEL electrophoresis  Sample fractionation  Snake venom  Walterinnesia aegyptia   
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