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Team:BYU Provo/Notebook/Cholera - Enzymes/Protocols
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| - | <font size="4"> ''' | + | <font size="4"> '''Synthetic Sea Water (SSW) LB recipe''' </font> |
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Fill to 1000 ml and autoclave | Fill to 1000 ml and autoclave | ||
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| + | <font size="4"> '''''V. cholerae'' Biofilm growth''' </font> | ||
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| + | Start a 5 ml overnight of ''V. cholerae'' in SSW LB and incubate at 30° for 72 hours. In a separate culture tube add 4 ml SSW LB and 50 ul overnight culture. Incubate at 30°C for at least 48 hours. | ||
<font size="4"> '''Phusion PCR (50ul reaction)''' </font> | <font size="4"> '''Phusion PCR (50ul reaction)''' </font> | ||
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<font size="4"> '''''V. cholerae'' Biofilm Degradation Assay''' </font> | <font size="4"> '''''V. cholerae'' Biofilm Degradation Assay''' </font> | ||
| - | + | *Revised from original Biofilm Degradation Assay from Pitts, B.; Hamilton, M.; Zelver, N.; Stewart, P. A Microtiter-Plate Screening Method for Biofilm Disinfection and Removal. J. Micro Methods 2003, 54, 269-276. ''V. cholerae'' biofilms are more apt to free float rather than develop on solid surfaces. | |
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| - | For each sample add 1 ml | + | For each sample add 1 ml SSW LB and 50 ul overnight seed. Add appropriate amount of degrading enzymes to each sample labeled ''time = 0 hours.'' Incubate at 30°C for 48. |
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===Any deviations from these protocols are listed in the notebook when they were used=== | ===Any deviations from these protocols are listed in the notebook when they were used=== | ||
Revision as of 22:28, 27 September 2013
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Cholera-Enzyme Protocols
Synthetic Sea Water (SSW) LB recipe
To 950 ml distilled H2O add
Adjust pH to 7.8
Fill to 1000 ml and autoclave
V. cholerae Biofilm growth
Start a 5 ml overnight of V. cholerae in SSW LB and incubate at 30° for 72 hours. In a separate culture tube add 4 ml SSW LB and 50 ul overnight culture. Incubate at 30°C for at least 48 hours. Phusion PCR (50ul reaction)
For each sample add:
Set the PCR machine to run the following cycle with the middle three phases being repeated 35 times
Hold at 4°C
Taq polymerase PCR (50ul reaction)
For each sample add:
Set the PCR machine to run the following cycle with the middle three phases being repeated 35 times
Hold at 4°C
Restriction Digest (50ul reaction)
For each sample add:
Place in 37°C incubator or water bath for 1.5 hours
Ligation
For each ligation reaction add
Incubate the reaction at room temperature for 30 minutes
Transformations
Set two heat blocks at 42°C and 37°C respectively. Thaw 25 ul of chemically competent cells on ice and add 5 ul of DNA to be cloned in. Place on ice for approximately 5 minutes. Heat shock at 42°C for 1 minute and immediately place back on ice for 2-5 minutes. Add 500 ul LB to the reaction and incubate at 37°C for 30 minutes. Plate 100 ul of cell on appropriate antibiotic plate and incubate at 37°C overnight.
V. cholerae Biofilm Degradation Assay
For each sample add 1 ml SSW LB and 50 ul overnight seed. Add appropriate amount of degrading enzymes to each sample labeled time = 0 hours. Incubate at 30°C for 48.
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