Team:UC Davis/Notebook

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== Week 4 ==
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--Monday 7/04/11--
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Happy 4th of July for all the Americans!  Today we started making more competent cells for the new strain BW22826.  Tomorrow we will complete the protocol.
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--Tuesday 7/05/11--
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BW22826 Cells had very fast growth overnight, and were too overgrown to use for competent cells in the morning. The procedure was restarted late at night (around 9:30) and lesser amounts of starter culture were used (1, 2, and 2 mL) to ensure the cells don't overgrow. One culture was placed on a shaker at room temperature, the other two were placed on a bench at room temperature.
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We inspected our LacI mutants. Most of the plates were covered in white colonies, though a few had some slightly pink colonies, indicating mutations were successful. The cells were plated on IPTG+ plates, so we expect induction; it is possible that the mutation rate was high and the promoter function was destroyed in a majority of colonies. Ten pink and ten white colonies were replated on IPTG+ plates, to rule out poor induction on our initial plates.
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E0240 variants with B0034 and with no RBS in pSB1K3 were cultured.
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--Wednesday 7/06/11--
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The making of our competent cells was successful! We were able to produce two full boxes today, with good amounts of cells in each of the tubes. Hopefully we won't have to make more for a while.
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We also miniprepped the E0240 variants from yesterday so that we could proceed with construction. We digested these minipreps along with our three main promoters (R0040, R0051, R0010) so that we could ligate them together.
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--Thursday 7/07/11--
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Today started slow but ended in a flurry!  We ligated three promoters (R0010, R0040, R0051) to E0240 (GFP) and transformed them.  We also retransformed our mutant LacI ligations to try and get even more.  The previous batch of potential mutants which were different shades of red on a replica plate got replated to see if we'll be able to see a clearer difference between shades of red on streaked plates.  So far there appears to be a good range of redness which is a positive sign that our mutagenic pcr worked somewhat well.  Out of 12 plates, we got 9 possible mutants.  We're planning on taking a closer look with our Tecan plate reader early next week.  This will give some more definitive proof of good mutants or not.  These mutants also got cultured so we can prepare them for sequencing soon. 
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In the Dh5α strain, LacI repressor is always present so, upon induction we expected to see red.  It seems from our mutation protocol that we mutated them too heavily since most colonies were white even with IPTG present. 
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--Friday 7/08/11--
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Mutated C0012, C0051, C0040. 
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Ligations of promoters to GFP looked green=good!
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Made control constructs for R0010
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Ligated R0040 and R0051 mutants into promoter screening plasmid for screening! 
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== Week 5 ==
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--Monday 7/11/11--
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While we are making and testing promoter mutants, we started making repressor mutants.  We'll need them eventually and the mutagenic PCR's don't take too long to do while things are slow.  However, testing out these mutants and finding a good range of repression is the tough part.  We also cut the wild-type repressors for construction of our testing plasmid. 
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--Tuesday 7/12/11--
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--Wednesday 7/13/11--
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<h3>Week Selection</h3>
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Finally got the Tecan set up how we want it for characterization of our mutants.  
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<td><a href="https://2011.igem.org/Team:UC_Davis/Notebook/Week_1">1</a></td>
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Miniprepped J61002 in a chloramphenicol backbone, this should come in handy later!
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<td><a href="https://2011.igem.org/Team:UC_Davis/Notebook/Week_2">2</a></td>
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<td><a href="https://2011.igem.org/Team:UC_Davis/Notebook/Week_3">3</a></td>
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Completely reorganized the 4 degree room. Now we can actually find our plates!
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<td><a href="https://2011.igem.org/Team:UC_Davis/Notebook/Week_4">4</a></td>
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<td><a href="https://2011.igem.org/Team:UC_Davis/Notebook/Week_5">5</a></td>
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--Thursday 7/14/11--
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<td><a href="https://2011.igem.org/Team:UC_Davis/Notebook/Week_6">6</a></td>
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<td><a href="https://2011.igem.org/Team:UC_Davis/Notebook/Week_7">7</a></td>
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Uh-oh! Our transformations from yesterday failed. Colonies on all of the controls! We're going to re-digest the following parts:
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<td><a href="https://2011.igem.org/Team:UC_Davis/Notebook/Week_8">8</a></td>
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<td><a href="https://2011.igem.org/Team:UC_Davis/Notebook/Week_9">9</a></td>
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* C0040 (Cut with XbaI and PstI)
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<td><a href="https://2011.igem.org/Team:UC_Davis/Notebook/Week_10">10</a></td>
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* C0012 (Cut with XbaI and PstI)
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<td><a href="https://2011.igem.org/Team:UC_Davis/Notebook/Week_11">11</a></td>
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* C0051 (Cut with XbaI and PstI)
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<td><a href="https://2011.igem.org/Team:UC_Davis/Notebook/Week_12">12</a></td>
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* C0051 (Cut with SpeI and PstI)
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<td><a href="https://2011.igem.org/Team:UC_Davis/Notebook/Week_13">13</a></td>
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* E0240 (Cut with XbaI and PstI)
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  <td><a href="https://2011.igem.org/Team:UC_Davis/Notebook/Week_14">14</a></td>
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* B0034 (Cut with SpeI and PstI)
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  <td><a href="https://2011.igem.org/Team:UC_Davis/Notebook/Week_15">15</a></td>
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  <td><a href="https://2011.igem.org/Team:UC_Davis/Notebook/Week_16">16</a></td>
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Set up PCR reactions in order to Gibson our project togetherThe parts PCR'd were c0012, C0051, C0040, I13458, I13453, E0240, R0010, R0051, and R0040Will see how they look on a gel and then Gibson them togetherSo many primers!
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Keegan took the GRE today!
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<h1>Notebook</h1>
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Welcome to our notebook. Here, you may will find summaries of our progress, pictures from throughout the summer, and information on the protocols we use in our lab.<br><br>
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--Friday 7/15/11--
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You may select a week above to travel directly to it, or begin at Week 1 <a href="https://2011.igem.org/Team:UC_Davis/Notebook/Week_1"><font style="color:#EE3333; size:40px;"> here</font></a>.
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If you're interested in what we've been up to since the first jamboree, you can see our progress <a href="https://2011.igem.org/Team:UC_Davis/Notebook/Post_American_Jamboree"><font style="color:#EE3333; size:40px;">here</font><a>.
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Today was a really fun day!  We did some minipreps in the morning but then drove down to UC Berkeley for a NorCal iGEM picnic.  We got to talk with our fellow iGEMers from UCSF and Berkeley and got updates on how their projects were going.  It was nice to see that there is a community of synthetic biologists in Northern California that we can share ideas and materials with.  After a relaxed lunch, we had a small meeting to discuss how to achieve the medal requirements.  We discussed helping each other to fulfill one of the gold medal requirements with the Berkeley team since some of our software tools might be useful for their project this year.  We then got to see their lab and received some pBAD+AraC since those parts from the registry seem to be faulty.  Overall a really good day!
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== Week 6 ==
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<h2>Gallery</h2>
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We have a ton of photos in our gallery that didn't end up being used elsewhere on the website, including a few that were too silly to post anywhere else. Check them out <a href="https://2011.igem.org/Team:UC_Davis/Gallery"><font style="color:#EE3333; size:40px;"> here</font></a>.<br><br>
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<h2>Protocols</h2>
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Looking for the mix for our mutagenic PCR protocol? Performing a ligation and you're not sure how much vector to use? Check out our <a href="https://2011.igem.org/Team:UC_Davis/Protocols"><font style="color:#EE3333; size:40px;"> Protocols</font></a> page for step-by-step instructions on how to replicate our experiments.<br>
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We weren't able to get all the parts for Gibson-ing our construct together.  We're still waiting on the 3 repressor PCRs and the pBAD promoter part.  The other's have been extracted and have decent concentrations for a Gibson mix.
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Today we transformed pBAD+AraC for PCRing tomorrow. 
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We also proceeded with the construction of our testing plasmid. We digested C0040, C0012, C0051 at XbaI and PstI so that we could ligate it into B0034, which we cut at SpeI and PstI. Additionally, we cut  all of our promoter-GFP parts at EcoRI and SpeI, so that we could ligate them with I13453, cut at EcoRI and XbaI. We ran them on a gel, purified them, and plan on ligating and transforming them tomorrow.
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--Tuesday --
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We ligated and transformed yesterday's gel purifications today. if this works, we'll be very close to finishing construction!
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--Wednesday --
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Strange! Our plates from yesterday are covered with lots of green colonies, even the parts that don't contain GFP! We're going to do some tests; perhaps our media is contaminated, or the water that was used for ligations. We will re-ligate these parts, and re-digest from the minipreps. We ran these re-digestions on gel in order to extract the segment we wanted, but noticed some odd things about the bands. In the lanes containing our vectors, there were three bands where we would expect to only see one. This indicated to us that there was likely some contamination before our digestion. We went ahead and transformed the re-ligated gel purifications from earlier this week.
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Took a picture of Nick. He wasn't too happy. We fixed it.
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--Thursday--
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Once again, our plates are contaminated with green colonies. After some deliberation, we believe that our old media was contaminated with GFP-containing bacteria, and that media was used to culture some of our parts prior to a miniprep. Those minipreps, then, have both plasmids. We're going to re-streak the parts from glycerol stocks, and make new minipreps.
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Aaron made the bench into an igloo today complete with dry ice effects.  
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We also re-transformed C0051+E0240. Let's hope it works this time.
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== Week 7 ==
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--Monday 7/25/11--
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We continued with construction today and, once again, extracted the cut Promoters+GFP and repressors from a gel. We ligated the promoters+GFP in from of I13453 and the repressors before B0034. Hopefully this is the last time we will have to ligate and transform these parts.
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--Tuesday 7/26/11--
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The insert controls for yesterday's transformations looked good, but there were still a good amount of colonies on the vector controls. We decided to do a PCR screen of these parts to make sure that they were the right length.
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Today was also "Tip Day"! We filled enough tip boxes to last us a quite a while.
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== Week 8 ==
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== Week 9 ==
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== Week 10 ==
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Latest revision as of 21:05, 28 October 2011

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Criteria

View our judging criteria for iGEM 2011 here.

Week Selection

1 2 3 4 5 6 7 8 9 10 11 12 13 14 15 16

Notebook

Welcome to our notebook. Here, you may will find summaries of our progress, pictures from throughout the summer, and information on the protocols we use in our lab.

You may select a week above to travel directly to it, or begin at Week 1 here.

If you're interested in what we've been up to since the first jamboree, you can see our progress here.

Protocols

Looking for the mix for our mutagenic PCR protocol? Performing a ligation and you're not sure how much vector to use? Check out our Protocols page for step-by-step instructions on how to replicate our experiments.