Difference between revisions of "Team:Aachen/Lab/Glycogen"
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<html><div class="col-md-12"></html> | <html><div class="col-md-12"></html> | ||
{{Team:Aachen/ReadMore|title=Characte-rization|link=/Team:Aachen/Lab/Glycogen/Characterization|picture=rmStaining}} | {{Team:Aachen/ReadMore|title=Characte-rization|link=/Team:Aachen/Lab/Glycogen/Characterization|picture=rmStaining}} | ||
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{{Team:Aachen/ReadMore|title=Glycogen Synthesis|link=/Team:Aachen/Lab/Glycogen/Synthesis|picture=rmGlycogenSynthesis|url=/wiki/images/9/97/Aachen_tile_Lab_Glycogen_Glycogen_synthesis.JPG}} | {{Team:Aachen/ReadMore|title=Glycogen Synthesis|link=/Team:Aachen/Lab/Glycogen/Synthesis|picture=rmGlycogenSynthesis|url=/wiki/images/9/97/Aachen_tile_Lab_Glycogen_Glycogen_synthesis.JPG}} | ||
− | <html></div></html> | + | <html></div><span style="color:transparent;line-heigth:0em;">a</span></html> |
+ | =Learn more= | ||
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When a bioprocess is developed in the lab, glucose is a popular choice for a carbon source. Even for industrial processes, sugars in general remain the number one substrate.<ref> Liu S. 2013. Bioprocess Engineering: Kinetics, Sustainability, and Reactor Design.</ref> | When a bioprocess is developed in the lab, glucose is a popular choice for a carbon source. Even for industrial processes, sugars in general remain the number one substrate.<ref> Liu S. 2013. Bioprocess Engineering: Kinetics, Sustainability, and Reactor Design.</ref> | ||
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While some processes will be adapted to methanol as the carbon source, most existing processes will still rely on sugars as these are well established and laborous to change. | While some processes will be adapted to methanol as the carbon source, most existing processes will still rely on sugars as these are well established and laborous to change. | ||
− | By converting renewable methanol to glycogen, the bacterial equivalent to starch, we will provide a [[Team:Aachen/Project/ | + | By converting renewable methanol to glycogen, the bacterial equivalent to starch, we will provide a [[Team:Aachen/Project/Background#Universal_carbon_source| universal carbon source]], connecting many existing bioprocesses to a sustainable substrate. |
==Our approach== | ==Our approach== | ||
− | To pave the way for an industrial process, we need to modify ''E. coli'' to produce high concentrations of glycogen. It has previously been shown that a knockout of one glycogen degradation enzyme leads to the accumulation of glycogen in the cells (Fig. 2)<ref> Alonso-Casaju´s Nora et al. 2006. Glycogen Phosphorylase, the Product of the glgP Gene, Catalyzes Glycogen Breakdown by Removing Glucose Units from the Nonreducing Ends in Escherichia coli</ref>. To further improve the production of glycogen in ''E. coli'', we approached this problem in our project in two ways: | + | To pave the way for an industrial process, we need to modify ''E. coli'' to produce high concentrations of glycogen. It has previously been shown that a knockout of one glycogen degradation enzyme leads to the accumulation of glycogen in the cells (Fig. 2) <ref name="sa"> Alonso-Casaju´s Nora et al. 2006. Glycogen Phosphorylase, the Product of the glgP Gene, Catalyzes Glycogen Breakdown by Removing Glucose Units from the Nonreducing Ends in Escherichia coli </ref>. To further improve the production of glycogen in ''E. coli'', we approached this problem in our project in two ways: |
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− | {{Team:Aachen/DoubleFigure|Aachen_glycogen metabolism adjusted.png|Aachen Glyogen accumulation of ∆glgP.png|title1= Figure 1 - Glycogen enzymes in ''E. coli'' |title2=Figure 2 - ∆''glgP'' ''E. coli'' cells|subtitle1=GlgC forms ADP-glucose from ATP and glucose-1-phosphate. The ADP-glucose is then used by GlgA which also serves as the starting particle through autophosphorylation. GlgB adds branches to the existing chains forming α-1,6-glycosidic bonds. GlgX degrades glycogen by cleaving α-1,6-glycosidic bonds whereas GlgP removes glucose units from the end of linear chains.|subtitle2= ''E. coli'' cells lacking ''glgP'' are shown. They accumulated glycogen in granules. By Alonso-Casaju´s Nora et al. 2006 <ref> Alonso-Casaju´s Nora et al. 2006. Glycogen Phosphorylase, the Product of the glgP Gene, Catalyzes Glycogen Breakdown by Removing Glucose Units from the Nonreducing Ends in Escherichia coli</ref>|size=large}} | + | {{Team:Aachen/DoubleFigure|Aachen_glycogen metabolism adjusted.png|Aachen Glyogen accumulation of ∆glgP.png|title1= Figure 1 - Glycogen enzymes in ''E. coli'' |title2=Figure 2 - ∆''glgP'' ''E. coli'' cells|subtitle1=GlgC forms ADP-glucose from ATP and glucose-1-phosphate. The ADP-glucose is then used by GlgA which also serves as the starting particle through autophosphorylation. GlgB adds branches to the existing chains forming α-1,6-glycosidic bonds. GlgX degrades glycogen by cleaving α-1,6-glycosidic bonds whereas GlgP removes glucose units from the end of linear chains.|subtitle2= ''E. coli'' cells lacking ''glgP'' are shown. They accumulated glycogen in granules. By Alonso-Casaju´s Nora et al. 2006 <ref name="sa"> Alonso-Casaju´s Nora et al. 2006. Glycogen Phosphorylase, the Product of the glgP Gene, Catalyzes Glycogen Breakdown by Removing Glucose Units from the Nonreducing Ends in Escherichia coli </ref>|size=large}} |
<span style="color:transparent">a</span> | <span style="color:transparent">a</span> |
Latest revision as of 00:48, 19 September 2015