Team:Calgary/Notebook/Protocols/potentiostatic
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- | <li>Grow cells overnight in 3mL of LB.</li> | + | <li><a href="https://2012.igem.org/Team:Calgary/Notebook/Protocols/onculture">Grow cells overnight</a> in 3mL of LB.</li> |
<li>Pellet cells at 3750rpm for 10 minutes.</li> | <li>Pellet cells at 3750rpm for 10 minutes.</li> | ||
<li>Remove the supernatant.</li> | <li>Remove the supernatant.</li> |
Latest revision as of 03:01, 4 October 2012
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Reporter Expression Detection
Similar to when creating a standard curve potentiostatically the working electrode must be held at a specific oxidation potential for the detection of that analyte. Testing for this requires a culture of cells that will be able to report through a hydrolase enzyme. To perform the detection a three electrode setup will be needed.
- Grow cells overnight in 3mL of LB.
- Pellet cells at 3750rpm for 10 minutes.
- Remove the supernatant.
- Resuspend in 1mL of 0.1M pH7 PBS.
- Add to 25mL 0.1M pH7 PBS in an electrochemical cell.
- Add the solution to be tested for activation of the reporter gene.
- Add the electrodes and close the cell.
- Insert a needle and bubble nitrogen or argon gas into the solution for 5 minutes.
- Hold the working electrode at the oxidation potential for the analyte product.
- Wait 5 minutes for current stabilization.
- Add the sugar-analyte substrate.
- Observe any current changes over a time period.
- Relate to the concentration of the analyte produced using a standard curve.