Team:Washington/Protocols/EG Assay
From 2012.igem.org
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=Turbidostat: Ethylene Glycol Assay= | =Turbidostat: Ethylene Glycol Assay= | ||
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+ | <li><b><font size="4">Turbidostat Preparation</font></b></li> | ||
<ol> | <ol> | ||
<li> Created M9 30mM ethylene glycol media</li> | <li> Created M9 30mM ethylene glycol media</li> | ||
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<li> Wait till program reads out optical density values - should see "0.000" as first optical density value</li> | <li> Wait till program reads out optical density values - should see "0.000" as first optical density value</li> | ||
</ol> | </ol> | ||
- | < | + | <li><b><font size="4">Cell Preparation</font></b><li> |
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<ol> | <ol> | ||
<li> Culture an overnight of MG1655 transformed with fucO pGA3K3 and aldA pGA1C3 in 2mL of TB with kanamycin and chloramphenicol</li> | <li> Culture an overnight of MG1655 transformed with fucO pGA3K3 and aldA pGA1C3 in 2mL of TB with kanamycin and chloramphenicol</li> | ||
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<li> Repeat steps 3-5 two more times </li> | <li> Repeat steps 3-5 two more times </li> | ||
</ol> | </ol> | ||
- | < | + | <li><b><font size="4">Turbidostat Inoculation and Operation</font></b></li> |
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<ol> | <ol> | ||
<li> Take a hypodermic needle attached to a 2.5mL syringe and aspirate 0.5mL of washed cells </li> | <li> Take a hypodermic needle attached to a 2.5mL syringe and aspirate 0.5mL of washed cells </li> | ||
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<li> Stop turbidostat program </li> | <li> Stop turbidostat program </li> | ||
<li> Retrieve data files from program folder and analyze them using your favorite mathematical software (ie: [http://www.mathworks.com/products/matlab/ Matlab] or [http://www.wolfram.com/mathematica/ Mathematica]</li> | <li> Retrieve data files from program folder and analyze them using your favorite mathematical software (ie: [http://www.mathworks.com/products/matlab/ Matlab] or [http://www.wolfram.com/mathematica/ Mathematica]</li> | ||
+ | </ol> | ||
</ol> | </ol> | ||
</html> | </html> |
Revision as of 00:14, 4 October 2012
Turbidostat: Ethylene Glycol Assay
- Turbidostat Preparation
- Created M9 30mM ethylene glycol media
- Sterile 200mL of 5X M9 salts
- 2.8mL of filter sterilized 99.99% ethylene glycol
- 800mL of sterile double distilled water
- Autoclave the the closed system of tubing, syringes, culture vessel, and empty bottle
- Wrap all open ends of the system with aluminium foil before autoclaving to prevent autoclave water from entering the closed tubing system
- Place closed system into the turbidostat apparatus
- Carefully and sterilely decant previously made sterile M9 30 mM ethylene glycol media into the media bottle
- Place turbidostat into a 37º C incubator
- Connect turbidostat to a computer with the turbidostat software and related libraries installed
- Start up turbidostat Program
-
- Be sure to close incubator door to reduce amount of ambient light
- Wait till program reads out optical density values - should see "0.000" as first optical density value
- Cell Preparation
-
- Culture an overnight of MG1655 transformed with fucO pGA3K3 and aldA pGA1C3 in 2mL of TB with kanamycin and chloramphenicol
- Take 1mL from the overnight culture and pipette it into a 1.5mL microcentrifuge tube
- Pellet the 1mL aliquot at 4000g for 3 minutes
- Pour out the supernatant
- Resuspend the pelleted cells with 1mL of sterile PBS
- Repeat steps 3-5 two more times
- Turbidostat Inoculation and Operation
- Take a hypodermic needle attached to a 2.5mL syringe and aspirate 0.5mL of washed cells
- Open incubator and through the soft stopper at the top of the culture vessel, inject the cells into the culture vessel to an OD ~0.2
- Close incubator door
- Wait 12-24 hours
- Stop turbidostat program
- Retrieve data files from program folder and analyze them using your favorite mathematical software (ie: [http://www.mathworks.com/products/matlab/ Matlab] or [http://www.wolfram.com/mathematica/ Mathematica]