Team:Sevilla/Week10
From 2011.igem.org
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<p>On the other hand, our constructions haven't arrived on time so we'll have to give up that option and stick to what we have now. We're having a bussy weekend: the parts must be sent next week and there's still a lot to do.LAST PUSH GUYS! | <p>On the other hand, our constructions haven't arrived on time so we'll have to give up that option and stick to what we have now. We're having a bussy weekend: the parts must be sent next week and there's still a lot to do.LAST PUSH GUYS! | ||
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<p> We're taking turns to get some sleep, but the floor is not exactly comfortable, and the cleaners come at 6 a.m... At least we have enough food to survive, a coffee machine and 4 litres of Coca-Cola. What a long weekend...</p> | <p> We're taking turns to get some sleep, but the floor is not exactly comfortable, and the cleaners come at 6 a.m... At least we have enough food to survive, a coffee machine and 4 litres of Coca-Cola. What a long weekend...</p> | ||
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Revision as of 22:45, 21 September 2011
Monday 12 September
One more week. We get to the lab in the morning. We open the incubator...
What the...FUCK? Honestly,is somebody kidding us? Where's the hidden camera? What the hells' wrong? Not a single colony in our transformation plates. AGAIN. Will it EVER work, for goodness sake? We've tried almost everything! Should we pray to God, to Superman, to Mr. Gibss?? Let's start again... :(
Tuesday 13 September
At least the boys are coming back little by little and we have more hands in the lab to work, and this is a bit more crowded and cheerful. We're starting to think more seriously about the Jamboree, there's still so much to do about the wiki, the parts, the team t-shirts, the flights, etc.
Wednesday 14 September
While we keep fighting against our naughty bacteria and the "standard" parts, we're also testing the biobrick T9002, developed by the Cambridge Lab in 2005. Ana is helping us to plan the experiments.
Wednesday Protocols
IMPROVED PROTOCOLS
Ligation
We are going to assemble small DNA fragments (inserts) with plasmids, so we will use bigger amount of inserts than os plasmid. Our ligation mix contains:
- 1 μL of 10X ligase buffer. It´s important to keep it on ice and also to resuspend it very well before using it. (Ligase buffer must contains ATP).
- 1 μL of ligase(It must be the last thing you add to the mix). You must not sink the tip too deep in order not to carry much glycerol. KEEP IT IN THE FREEZER, even when you use it.
- 1 or 2 μL of plasmid.
- 7 or 6 μL of insert.
Keep at room temperature overnight.
Double Digestion
20 μL must be the final volumen of our digestion mix. We must add:
- 2 μL of buffer
- 0,5 μL of each enzyme (We use EcorI, SpeI, XbaI and PstI). This amount of enzyme must be individually determine depending on the amunt of DNA you are going to digest
- 16 μL of Milli-Q water
- 1 μL of DNA sample
It´s important that you shake the mixture using the centriguge. 1 minute at medium speed must works.
Transformtion
1. In the same tube, mix:
- 25 μL of competent cells.
- 1 μL of DNA sample (the amount of DNA depends on the concentration of your sample)if yor DNA is pure. If not, use aproximately 3 μL.
*Use very cold pipets.
2. Incubate the tube on ice for 30 minutes.
3. Incubate at 42ºC for 30 seconds.
4. Incubete 2 minutes on ice for 2 minutes.p>
5. Add 225 μL of NZY, LB, or SOB (preheated in the 42 degrees bath). You must add 225 μL of medium culture per each microlitre of DNA sample you use.
6. Keep the tube for 45 minutes or 1h in agitacion at 37ºC
**If you are using complex DNA ligations for the transformation, you must add beta-mercaptoethanol before the half an hour incubation on ice
Thursday 15 September
Ligation 1 has grown!!!! Isn't it incredible? It's a fusion of F2620 and I732019, it should be able to sense C6-3-oxo-HSL in the media and express lacZ as a reporter. We'll have to make a liquid culture to get the plasmid tomorrow, digest it to check if the insert has the appropiate length and see if it works. For the last part, we seed the bacteria in a plate with the signal and XGal that should turn blue when lacZ is expressed.
Friday 16 September
YEAAAAAAAAAH! IT WORKS!!! Look at this plate and the little blue spots! IT WORKS! Sadly,we have to digest the plasmid, extract the insert and place it in pSB1C3, because now it's in pSB1A2. Let's hope this time the cycle works as it should.
On the other hand, our constructions haven't arrived on time so we'll have to give up that option and stick to what we have now. We're having a bussy weekend: the parts must be sent next week and there's still a lot to do.LAST PUSH GUYS!
Weekend
Marathon weekend doing mini-preps of every single colony we have, with their restrictions, electrophoresis, purification, etc. This means more than 30 digestions ONLY for one construction. Besides, we're also working with some of the other planned constructions, and we're doing everything in duplicate to try different protocols in line. We're running out of time,and the electrophoresis machinery is smoking. We're using two different competent cells, kipping the ligationsat different temperatures at different times...We have to try everything!
We're taking turns to get some sleep, but the floor is not exactly comfortable, and the cleaners come at 6 a.m... At least we have enough food to survive, a coffee machine and 4 litres of Coca-Cola. What a long weekend...