Difference between revisions of "Team:UMaryland/Protocols"
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| − | -Prepare multi well plate containing serial dilutions of concentrated PCA solution in wells. Fill gaps between wells with water to prevent drying. Fill wells on edges with water. | + | -Prepare multi well plate containing serial dilutions of concentrated PCA solution (in Tris buffer) in wells. Fill gaps between wells with water to prevent drying. Fill wells on edges with water. |
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- Optional: spin down plate and resuspend wells in PBS for reduced error | - Optional: spin down plate and resuspend wells in PBS for reduced error | ||
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| + | PcaU fluorescence to measure [TPA] | ||
| + | </div> | ||
| + | <div class="meatMeat"> | ||
| + | -Prepare multi well plate containing serial dilutions of concentrated TPA solution (in tris buffer) in wells. Fill gaps between wells with water to prevent drying. Fill wells on edges with water. | ||
| + | </div> | ||
| + | <div class="meatMeat"> | ||
| + | -Add TPH enzyme mix to each well and incubate at 30C overnight. Recommended 1 volume mix per 10 volumes total | ||
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| + | -When OD600 = 0.6-0.8, transfer a fixed volume of culture from the flask to each well except for the water wells on edges | ||
| + | </div> | ||
| + | <div class="meatMeat"> | ||
| + | -Proceed to protocol: PcaU fluorescence to measure [PCA] | ||
| + | </div> | ||
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Revision as of 16:13, 17 October 2018
Protocols
Lysing cells and using PCAU
PcaU fluorescence to measure [PCA]
-Culture BL21 E. coli containing PcaU fluorescent reporter in 50mL flask, 30C, 250rpm
-Prepare multi well plate containing serial dilutions of concentrated PCA solution (in Tris buffer) in wells. Fill gaps between wells with water to prevent drying. Fill wells on edges with water.
-When OD600 = 0.6-0.8, transfer a fixed volume of culture from the flask to each well except for the water wells on edges
-Incubate >6 hours
- Read fluorescence in plate reader at 395 excitation 509 emission
- Optional: spin down plate and resuspend wells in PBS for reduced error
PcaU fluorescence to measure [TPA]
-Prepare multi well plate containing serial dilutions of concentrated TPA solution (in tris buffer) in wells. Fill gaps between wells with water to prevent drying. Fill wells on edges with water.
-Add TPH enzyme mix to each well and incubate at 30C overnight. Recommended 1 volume mix per 10 volumes total
-When OD600 = 0.6-0.8, transfer a fixed volume of culture from the flask to each well except for the water wells on edges
-Proceed to protocol: PcaU fluorescence to measure [PCA]
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umarylandigem@gmail.com
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