Difference between revisions of "Part:BBa K801080:Experience"
(Undo revision 149127 by Fabian Froehlich (Talk)) |
(Undo revision 149125 by Fabian Froehlich (Talk)) |
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===Expression of Thaumatin=== | ===Expression of Thaumatin=== | ||
+ | [[File:celllysate_thaumatin_sdspage_TUM12.jpg|right|312px]] | ||
+ | The BioBrick for Thaumatin in our yeast vector pTUM104 was expressed in YPD media in a 2l scale and the cells were harvested and disrupted using glass beads. On the SDS-Page showing the cell lysate there was no additional band at the size of Thaumatin. | ||
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+ | We plan to do a western blot of the supernatant to prove proper secretion. SDS page and coomassie/silver staining have proven to be too insensitive. | ||
+ | <div style="clear:both"> | ||
==== Ion exchange chromatography ==== | ==== Ion exchange chromatography ==== | ||
</div> | </div> | ||
− | [[file:TUM12_ThaumatinIEC.png|500px|thump|right| | + | [[file:TUM12_ThaumatinIEC.png|500px|thump|right|Bildbeschreibung]] |
Preprothaumatin becomes posttranslationally modified by cleaving a part of the N- and the C-terminal polypeptide. Therefore it was not possible to add a tag for affinity chromatography. For this reason it was necessary to purify the protein from the cytoplasm of the desintegrated yeast cells using ion exchange chromatography to have a proove of principle. | Preprothaumatin becomes posttranslationally modified by cleaving a part of the N- and the C-terminal polypeptide. Therefore it was not possible to add a tag for affinity chromatography. For this reason it was necessary to purify the protein from the cytoplasm of the desintegrated yeast cells using ion exchange chromatography to have a proove of principle. | ||
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Expression of ThaumatinThe BioBrick for Thaumatin in our yeast vector pTUM104 was expressed in YPD media in a 2l scale and the cells were harvested and disrupted using glass beads. On the SDS-Page showing the cell lysate there was no additional band at the size of Thaumatin.
Ion exchange chromatographyPreprothaumatin becomes posttranslationally modified by cleaving a part of the N- and the C-terminal polypeptide. Therefore it was not possible to add a tag for affinity chromatography. For this reason it was necessary to purify the protein from the cytoplasm of the desintegrated yeast cells using ion exchange chromatography to have a proove of principle. Experimental details:
Experimental results:
Conclusion from this experiment: |
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