EPF-Lausanne/10 October 2009
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==Wet Lab== | ==Wet Lab== | ||
+ | '''All cultures have grown''' | ||
- | + | '''IPTG stock solution''' | |
+ | |||
+ | 200 mM (for induction at 2 mM -> 100x) in 15 ml, so 0.714 g. | ||
+ | |||
+ | |||
+ | '''Setting the conditions for the culture:''' | ||
+ | |||
+ | Different conditions : | ||
+ | |||
+ | - + light / + IPTG / - TRP | ||
+ | |||
+ | - + light / - IPTG / - TRP | ||
+ | |||
+ | - - light / + IPTG / - TRP | ||
+ | |||
+ | - - light / - IPTG / - TRP | ||
+ | |||
+ | - - light / - IPTG / + TRP | ||
+ | |||
+ | Each condition for RO2.4 + BB1 /#3 DH5a LB and for RO1.1 + BB1/#1 DH5a LB. | ||
+ | |||
+ | Pre-prepared stock to aliquot : 3.5 ml of corresponding culture in 27 ml of new fresh LB (+ antibiotic). Flasks : +/- IPTG - trp, - IPTG + trp. Induction : TRP : 0.9 mg/ml, ITPG : 2 mM. Then we put the aliquot in eppendorf tubes (1ml). | ||
+ | |||
+ | Measurements : with abs/fluo on plate reader. | ||
+ | |||
+ | Each time a plate is prepared, the corresponding aliquot is used once only. | ||
+ | |||
+ | We put 200 ul in each well. | ||
+ | |||
+ | One plate served twice (2nd time the non-used wells were used). | ||
+ | |||
+ | ===pPCR experiment=== | ||
+ | Reinoculate 3 mL in 100 L, 900 ul of cells. | ||
+ | |||
+ | RO1 : only, + TRP, + TRP 2/3, +TRP 1/3. | ||
+ | |||
+ | RO2 : only, + TRP, + TRP 2/3, + TRP 1/3, + ATC, + ATC 1/2, LB only. | ||
+ | |||
+ | TRP : 1x corresponds to 100ul, 2/3 to 67 ul and 1/3 to 33 ul. | ||
+ | |||
+ | ATC : 1x corresponds to 20 ul in 180 ul LB so 100 ng/uL, 1/2 to 50 ng/ul (10 ul of ATC added in 90 ul LB). | ||
+ | |||
+ | Total in each well : 30 ul. | ||
+ | |||
+ | ===Kinetic experiment== | ||
+ | Observe the degradation of RFP over time with the plate reader. Observation on RO2.4 + BB1 and RO1.1 + BB1. | ||
+ | |||
+ | For each clone, 2 conditions : + IPTG / + light, - IPTG / - light. | ||
+ | |||
+ | ===Transformation=== | ||
+ | Making RO2 + BB and RO1 + BB in JRG 465 / JRG 1046. | ||
+ | |||
+ | 50 ul of cells : | ||
+ | |||
+ | RO2 + BB : 5 ul of the minipreped double transformants (containing both RO2.4 + BB1 /#3). Conc : 450 ng/ul. | ||
+ | |||
+ | RO1 + BB : 4 ul of RO1.1 at 154 ng/ul and 2.5 ul of BB1 at 250 ng/ul. | ||
==People in the lab== | ==People in the lab== |
Revision as of 11:57, 11 October 2009
Wet Lab
All cultures have grown
IPTG stock solution
200 mM (for induction at 2 mM -> 100x) in 15 ml, so 0.714 g.
Setting the conditions for the culture:
Different conditions :
- + light / + IPTG / - TRP
- + light / - IPTG / - TRP
- - light / + IPTG / - TRP
- - light / - IPTG / - TRP
- - light / - IPTG / + TRP
Each condition for RO2.4 + BB1 /#3 DH5a LB and for RO1.1 + BB1/#1 DH5a LB.
Pre-prepared stock to aliquot : 3.5 ml of corresponding culture in 27 ml of new fresh LB (+ antibiotic). Flasks : +/- IPTG - trp, - IPTG + trp. Induction : TRP : 0.9 mg/ml, ITPG : 2 mM. Then we put the aliquot in eppendorf tubes (1ml).
Measurements : with abs/fluo on plate reader.
Each time a plate is prepared, the corresponding aliquot is used once only.
We put 200 ul in each well.
One plate served twice (2nd time the non-used wells were used).
pPCR experiment
Reinoculate 3 mL in 100 L, 900 ul of cells.
RO1 : only, + TRP, + TRP 2/3, +TRP 1/3.
RO2 : only, + TRP, + TRP 2/3, + TRP 1/3, + ATC, + ATC 1/2, LB only.
TRP : 1x corresponds to 100ul, 2/3 to 67 ul and 1/3 to 33 ul.
ATC : 1x corresponds to 20 ul in 180 ul LB so 100 ng/uL, 1/2 to 50 ng/ul (10 ul of ATC added in 90 ul LB).
Total in each well : 30 ul.
=Kinetic experiment
Observe the degradation of RFP over time with the plate reader. Observation on RO2.4 + BB1 and RO1.1 + BB1.
For each clone, 2 conditions : + IPTG / + light, - IPTG / - light.
Transformation
Making RO2 + BB and RO1 + BB in JRG 465 / JRG 1046.
50 ul of cells :
RO2 + BB : 5 ul of the minipreped double transformants (containing both RO2.4 + BB1 /#3). Conc : 450 ng/ul.
RO1 + BB : 4 ul of RO1.1 at 154 ng/ul and 2.5 ul of BB1 at 250 ng/ul.
People in the lab
Christian, Heidi, Basile