Team:Paris Saclay/Notebook/August/22
From 2014.igem.org
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+ | ====PCR purification==== | ||
+ | We use the kit PCR clean-up | ||
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+ | the elution volume is 20µl | ||
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|Phusion | |Phusion |
Revision as of 10:28, 26 August 2014
Contents |
Friday 22nd August
Lab work
D - Lemon Scent
pPSI digestion
components | volumes |
---|---|
pPSI | 40μl |
FastDigest green buffer 10X | 5μl |
PacI | 2µl |
H2O | 2µl |
pPSI dephosphorylation
After 2 hours, add 1.5µL of Alkaline Phosphatase (AP) and let it 1 hour.
Then, inactivation of AP at 65°C during 15 minutes.
We've made a electrophoresis to check the digestion.
Legend
- pPSI+Apra digested via PacI, dephosphorylated 5µl
- pPSI+Apra digested via PacI, dephosphorylated 5µl
- ladder 5µl
Ligation of BBa_K517003, BBa_K762100, and Geraniol synthase in pPSI
components | volumes |
---|---|
BBa_K517003 | 10μl |
pPSI | 2μl |
buffer | 2µl |
H2O | 5µl |
ligase | 1µl |
components | volumes |
---|---|
BBa_K762100 | 10μl |
pPSI | 2μl |
buffer | 2µl |
H2O | 5µl |
ligase | 1µl |
components | volumes |
---|---|
GS | 10μl |
pPSI | 2μl |
buffer | 2µl |
H2O | 5µl |
ligase | 1µl |
And let it in the freezer for 3 hours.
Transformation in competent E.coli DH5α
After 3 hours, take out the ligation tubes and add 100 µl of competent DH5α in each tube.
Then proceed to the transformation protocol.
- 20 minutes at 4°C
- 2 minutes 30 seconds at 42°C
- 2 minutes at 4 °C
- Add 0.9 ml of LB into the tubes
Finally put it in a incubator at 37°C for 30 minutes
PCR of CAD
With or synthetic gene, we decided to do a PCR to have more matrice.
components | volumes |
---|---|
H2O | 27μl |
5x phusion buffer | 2µl |
dNTP 10 mM | 2µl |
iPS83 10µM | 5µl |
iPS84 10µM | 5µl |
DMSO | 1.5µl
PCR purificationWe use the kit PCR clean-up the elution volume is 20µl
|
Phusion | 0.5µl |
Temperature (°C) | time |
---|---|
98 | 30 sec |
98 | 10 sec |
58 | 30 sec |
72 | 45 sec |
72 | 10 min |