Team:Osaka/Protocols
From 2011.igem.org
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== Protocols == | == Protocols == | ||
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#Add mitomycin C to desired final concentration (we used 2µg/ml) and incubate at 37°C for a further 2h. | #Add mitomycin C to desired final concentration (we used 2µg/ml) and incubate at 37°C for a further 2h. | ||
#Centrifuge, discard mitomycin C-spiked medium and resuspend with fresh LB medium. | #Centrifuge, discard mitomycin C-spiked medium and resuspend with fresh LB medium. | ||
- | #[RECOMMENDED]Dilute pre-culture samples according to expected survival rate, as determined from a preliminary experiment (lower dilution rate is needed if fewer cells are expected to survive). | + | #[RECOMMENDED] Dilute pre-culture samples according to expected survival rate, as determined from a preliminary experiment (lower dilution rate is needed if fewer cells are expected to survive). |
- | # | + | #Pipette 50μl to LB agar plates and spread evenly. Air-dry the plates to remove excess wetness. |
#Wrap plates in aluminium foil and incubate at 37°C. | #Wrap plates in aluminium foil and incubate at 37°C. | ||
- | #After 16h, count number of colonies formed on control | + | #After 16h, count number of colonies formed on control and mitomycin C-treated inoculum plates. |
- | === SOS | + | |
+ | === SOS promoter assay 1: Carotenoid biosynthesis === | ||
#Pre-culture transformed cells in 8ml of LB medium at 37°C for 12h. | #Pre-culture transformed cells in 8ml of LB medium at 37°C for 12h. | ||
#Transfer pre-culture to OD600 measurement dish (ø50mm). | #Transfer pre-culture to OD600 measurement dish (ø50mm). | ||
#Irradiate with UV light at desired energy dosage. | #Irradiate with UV light at desired energy dosage. | ||
#Incubate irradiated cells for a further 2h. | #Incubate irradiated cells for a further 2h. | ||
- | #Measure OD600 as a | + | #Measure OD600 as a surrogate for cell density. |
#Transfer cells into 15ml Falcon tubes and centrifuge. | #Transfer cells into 15ml Falcon tubes and centrifuge. | ||
#Discard supernatant, add 1ml water to wash cells. | #Discard supernatant, add 1ml water to wash cells. | ||
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#Add 500μl acetone and vortex. | #Add 500μl acetone and vortex. | ||
#Incubate at 55°C for 15min. | #Incubate at 55°C for 15min. | ||
- | #Measure absorbance at 474nm. Use 100% acetone as blanks, and divide absorbances by OD600 | + | #Measure absorbance at 474nm. Use 100% acetone as blanks, and divide absorbances by OD600 values. |
+ | |||
+ | |||
+ | === SOS promoter assay 2: GFP === | ||
+ | #Pre-culture transformed cells in 20ml of LB medium at 37°C for 12h. | ||
+ | #Transfer pre-culture to OD600 measurement dish (ø50mm). | ||
+ | #Irradiate with UV light at desired energy dosage. | ||
+ | #Incubate irradiated cells for a further 2h. | ||
+ | #Measure OD600 as a surrogate for cell density. | ||
+ | #Transfer cells into 50ml Falcon tubes and centrifuge. | ||
+ | #Discard supernatant, add 4ml water to wash cells. | ||
+ | #Repeat centrifugation and decantation. | ||
+ | #Resuspend cells in 4ml water. | ||
+ | #Measure fluorescence at 395nm excitation and 509nm emission. Use pure water as blanks, and divide emission values by OD600 values. | ||
</div> | </div> |
Latest revision as of 23:45, 28 October 2011
Protocols
Cell survival assay 1: UV irradiation
- Pre-culture transformed cells in 3ml of LB medium at 37°C for 16h.
- Induce parts with IPTG addition (to final concentration of 100µM) for 1h.
- Dilute pre-culture samples according to intended UV energy dosage (if dosage is high, lower dilution rate is needed as fewer cells are expected to survive).
- Transfer 50μl of diluted pre-culture onto LB agar plates and spread evenly. Air-dry the plates to remove excess wetness.
- Irradiate cells on the agar with UV light at desired energy dosage.
- Wrap plates in aluminium foil and incubate at 37°C.
- After 16h, count number of colonies formed on control (non-irradiated) and UV-irradiated plates.
Cell survival assay 2: Mitomycin C
- Pre-culture transformed cells in 3ml of LB medium at 37°C for 16h.
- Induce parts with IPTG addition to final concentration of 100µM and incubate for 1h.
- Add mitomycin C to desired final concentration (we used 2µg/ml) and incubate at 37°C for a further 2h.
- Centrifuge, discard mitomycin C-spiked medium and resuspend with fresh LB medium.
- [RECOMMENDED] Dilute pre-culture samples according to expected survival rate, as determined from a preliminary experiment (lower dilution rate is needed if fewer cells are expected to survive).
- Pipette 50μl to LB agar plates and spread evenly. Air-dry the plates to remove excess wetness.
- Wrap plates in aluminium foil and incubate at 37°C.
- After 16h, count number of colonies formed on control and mitomycin C-treated inoculum plates.
SOS promoter assay 1: Carotenoid biosynthesis
- Pre-culture transformed cells in 8ml of LB medium at 37°C for 12h.
- Transfer pre-culture to OD600 measurement dish (ø50mm).
- Irradiate with UV light at desired energy dosage.
- Incubate irradiated cells for a further 2h.
- Measure OD600 as a surrogate for cell density.
- Transfer cells into 15ml Falcon tubes and centrifuge.
- Discard supernatant, add 1ml water to wash cells.
- Repeat centrifugation and decantation.
- Add 500μl acetone and vortex.
- Incubate at 55°C for 15min.
- Measure absorbance at 474nm. Use 100% acetone as blanks, and divide absorbances by OD600 values.
SOS promoter assay 2: GFP
- Pre-culture transformed cells in 20ml of LB medium at 37°C for 12h.
- Transfer pre-culture to OD600 measurement dish (ø50mm).
- Irradiate with UV light at desired energy dosage.
- Incubate irradiated cells for a further 2h.
- Measure OD600 as a surrogate for cell density.
- Transfer cells into 50ml Falcon tubes and centrifuge.
- Discard supernatant, add 4ml water to wash cells.
- Repeat centrifugation and decantation.
- Resuspend cells in 4ml water.
- Measure fluorescence at 395nm excitation and 509nm emission. Use pure water as blanks, and divide emission values by OD600 values.