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EPF-Lausanne/8 October 2009
From 2009.igem.org
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===Gel=== | ===Gel=== | ||
Here the 2nd strains seems to have a double transformant. But we let the gel overnight so there is no BrEth any more, we had to take a time of exposure of 38.2 s to see something. We will do a nicer gel this afternoon. | Here the 2nd strains seems to have a double transformant. But we let the gel overnight so there is no BrEth any more, we had to take a time of exposure of 38.2 s to see something. We will do a nicer gel this afternoon. | ||
| + | |||
| + | ===Preparation of the time-course experiment=== | ||
| + | The idea is to look at the evolution of fluorescence over the time, for different time of exposition on the light. | ||
| + | |||
| + | 7 ml of LB + 1 ml of DH5a RO2.4 + BB1 #3 overnight culture. | ||
| + | |||
| + | 5 conditions : | ||
| + | |||
| + | - + light + IPTG - Trp | ||
| + | |||
| + | - + light - IPTG - Trp | ||
| + | |||
| + | - - light + IPTG - Trp | ||
| + | |||
| + | - - light - IPTG + Trp | ||
| + | |||
| + | - - light - IPTG + Trp | ||
| + | |||
| + | - - light - IPTG - Trp | ||
| + | |||
| + | IPTG at 1 mM (100 mM sol. diluted 1/100). Trp diluted 1/25. Incubated in conditions at 37°C. Measures will be taken with plate reader every 30 minutes starting at 1h. | ||
| + | |||
| + | ===Miniprep=== | ||
| + | We did a miniprep of new strain double transformants to confirm gel results by digestion assay : | ||
| + | |||
| + | - RO1.1 + BB1 JRG 1046 (n°1,3,7) | ||
| + | |||
| + | - RO2.4 + BB1 JRG 1046 (n°1,3,6) | ||
| + | |||
| + | + miniprep of DH5 a RO2.4 + BB1 #3 (strain that works) to have the 2 plasmids for subsequent transformations. | ||
| + | |||
| + | ===Digestion assay=== | ||
| + | For each clones, we use digestion by P and S (since LovTAP contains 2 P sites and Trp op contains 2 S sites). For reaction, incubate at 37°C (INCUB37). Digestion of about 1h30. | ||
| + | |||
| + | ===Gel=== | ||
| + | Once again to see the double transformants + of digestion assay. | ||
==People in the lab== | ==People in the lab== | ||
Revision as of 07:20, 8 October 2009
Contents |
Wet Lab
Colony PCR
On the same double transformants -> 2 min extension.
Gel
Here the 2nd strains seems to have a double transformant. But we let the gel overnight so there is no BrEth any more, we had to take a time of exposure of 38.2 s to see something. We will do a nicer gel this afternoon.
Preparation of the time-course experiment
The idea is to look at the evolution of fluorescence over the time, for different time of exposition on the light.
7 ml of LB + 1 ml of DH5a RO2.4 + BB1 #3 overnight culture.
5 conditions :
- + light + IPTG - Trp
- + light - IPTG - Trp
- - light + IPTG - Trp
- - light - IPTG + Trp
- - light - IPTG + Trp
- - light - IPTG - Trp
IPTG at 1 mM (100 mM sol. diluted 1/100). Trp diluted 1/25. Incubated in conditions at 37°C. Measures will be taken with plate reader every 30 minutes starting at 1h.
Miniprep
We did a miniprep of new strain double transformants to confirm gel results by digestion assay :
- RO1.1 + BB1 JRG 1046 (n°1,3,7)
- RO2.4 + BB1 JRG 1046 (n°1,3,6)
+ miniprep of DH5 a RO2.4 + BB1 #3 (strain that works) to have the 2 plasmids for subsequent transformations.
Digestion assay
For each clones, we use digestion by P and S (since LovTAP contains 2 P sites and Trp op contains 2 S sites). For reaction, incubate at 37°C (INCUB37). Digestion of about 1h30.
Gel
Once again to see the double transformants + of digestion assay.
People in the lab
Heidi, Gab, Tu
