Difference between revisions of "Team:Virginia/Experiments"
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<b>Methods:</b><br> | <b>Methods:</b><br> | ||
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<button data-toggle="collapse" data-target="#pdtransformation">Transformation via Electroporation</button> | <button data-toggle="collapse" data-target="#pdtransformation">Transformation via Electroporation</button> | ||
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<li>1. Thaw and mix 50 uL portions cells with 5 uL DNA | <li>1. Thaw and mix 50 uL portions cells with 5 uL DNA | ||
<li>2. Transfer to ice cold electroporation cuvette | <li>2. Transfer to ice cold electroporation cuvette | ||
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<h2>Measurement protocols</h2> | <h2>Measurement protocols</h2> | ||
<button data-toggle="collapse" data-target="#promotercharacterization">Mn-Sod, VhB and T7 Promoter Characterization</button> | <button data-toggle="collapse" data-target="#promotercharacterization">Mn-Sod, VhB and T7 Promoter Characterization</button> | ||
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<b>Isolate Single colonies</b> | <b>Isolate Single colonies</b> | ||
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<button data-toggle="collapse" data-target="#ammoniumconversion">Measuring Efficiency of Ammonium Conversion and Nitrate Production Over Time | <button data-toggle="collapse" data-target="#ammoniumconversion">Measuring Efficiency of Ammonium Conversion and Nitrate Production Over Time | ||
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Revision as of 03:33, 1 November 2017
Protocols
Pc. denitrificans Protocols
Methods:
- Grow Pc. denitrificans cultures in liquid media
- Dilute 500mL of Pc. denitrificans culture in 500mL SGM17 medium
- ***Cold Room from here on***
- Harvest by centrifuge 250mL samples each in four centrifuge bottles at 5000xg at 4 C. carefully dump out supernatant
- Completely resuspend the pellets(shake side to side to avoid liquid loss) in all centrifuge bottles each with 50mL of 0.5 M sucrose solution with 10% glycerol
- Combine the liquid(containing resuspended pellets) into one centrifuge bottle, add appropriate amount of water to the other empty centrifuge bottle for counterbalance
- Centrifuge the two bottles at 5000xg at 4 C
- Dump out supernatant and resuspend the pellets with 100mL of 0.5 M sucrose solution with 10% glycerol. Counter-balance bottle should have 100mL of water
- Centrifuge the two bottles at 5000xg at 4 C
- Dump out supernatant and resuspend the resulting pellets in 10mL of 0.5 M sucrose solution with 10% glycerol
- Aliquot the final 10mL of liquid into 0.25mL(250uL) with 40 microcentrifuge tubes
- Flash freeze with liquid nitrogen and store at -80 C
Measurement protocols
Isolate Single colonies
Preculture for Device Testing
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