Team:DTU-Denmark/Notebook
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<title>Welcome to the DTU iGEM wiki!</title> | <title>Welcome to the DTU iGEM wiki!</title> | ||
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<td align="center" ><font face="arial" size="3"><a class="mainLinks" href="https://2010.igem.org/Team:DTU-Denmark/Project" >The Project</a> </font></td> | <td align="center" ><font face="arial" size="3"><a class="mainLinks" href="https://2010.igem.org/Team:DTU-Denmark/Project" >The Project</a> </font></td> | ||
<td align="center" ><font face="arial" size="3"><a class="mainLinks" href="https://2010.igem.org/Team:DTU-Denmark/Parts" >Parts submitted</a> </font></td> | <td align="center" ><font face="arial" size="3"><a class="mainLinks" href="https://2010.igem.org/Team:DTU-Denmark/Parts" >Parts submitted</a> </font></td> | ||
- | <td align="center" ><font face="arial" size="3"><a class="mainLinks" href="https://2010.igem.org/Team:DTU-Denmark/ | + | <td align="center" ><font face="arial" size="3"><a class="mainLinks" href="https://2010.igem.org/Team:DTU-Denmark/Results">Results</a></font> </td> |
<td align="center" ><font face="arial" size="3"><a class="mainLinks" href="https://2010.igem.org/Team:DTU-Denmark/Notebook" title="Day to day lab activity">Notebook</a> | <td align="center" ><font face="arial" size="3"><a class="mainLinks" href="https://2010.igem.org/Team:DTU-Denmark/Notebook" title="Day to day lab activity">Notebook</a> | ||
<td align="center" ><font face="arial" size="3"><a class="mainLinks" href="https://2010.igem.org/Team:DTU-Denmark/Blog">Blog</a></font> </td> | <td align="center" ><font face="arial" size="3"><a class="mainLinks" href="https://2010.igem.org/Team:DTU-Denmark/Blog">Blog</a></font> </td> | ||
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<ul type="circle"> | <ul type="circle"> | ||
- | <li><a href="https://2010.igem.org/Team:DTU-Denmark/ | + | <li><a href="https://2010.igem.org/Team:DTU-Denmark/Lab_protocols">Lab Protocols</a> |
- | <li><a href="https://2010.igem.org/Team:DTU-Denmark/Lab_protocols"> | + | <ul> |
+ | <font size="2"> | ||
+ | <li><a href="https://2010.igem.org/Team:DTU-Denmark/Lab_protocols#BioLector">BioLector</a></li> | ||
+ | <li><a href="https://2010.igem.org/Team:DTU-Denmark/Lab_protocols#Ligations">Ligations</a></li> | ||
+ | <li><a href="https://2010.igem.org/Team:DTU-Denmark/Lab_protocols#PCR_purification">PCR product purification</a></li> | ||
+ | <li><a href="https://2010.igem.org/Team:DTU-Denmark/Lab_protocols#Plasmid_purifcation">Plasmid purification by miniprep</a></li> | ||
+ | <li><a href="https://2010.igem.org/Team:DTU-Denmark/Lab_protocols#Restriction_Digestion">Restriction/Digestion</a></li> | ||
+ | <li><a href="https://2010.igem.org/Team:DTU-Denmark/Lab_protocols#Transformation ">Transformation </a></li> | ||
+ | </font></ul> | ||
+ | </li><br> | ||
+ | <li><a href="https://2010.igem.org/Team:DTU-Denmark/BioLector">BioLector</a></li><br> | ||
+ | <li><a href="https://2010.igem.org/Team:DTU-Denmark/Safety_considerations">Safety Considerations</a></li><br> | ||
</ul> | </ul> | ||
</td> | </td> | ||
<td> | <td> | ||
<h2>October</h2> | <h2>October</h2> | ||
+ | <h3>23-10-2010-Maya-Repressor group</h3> | ||
+ | <p align="justify"> Yesterday Sebastien transformed pIGR06 into a Salmonella strain to test whether the antirepressor works. Today I induced the pBAD promoter, which is infront of the antirepressor, by adding arabinose. After one hour I could see that the cells carrying the antirepressor-plasmid (pIGR06) lysed. This means that the antirepressor works:-) <br> | ||
+ | |||
+ | We tried once more to verify pIGR12, but the bands we got had really weird sizes.<br> | ||
+ | |||
+ | We also made the cells carrying pIGR03 and pIGR04 competent, and transformed pIGR05 and pIGR06 into these. <br></p> | ||
+ | |||
+ | <h3> 22-10-2010-Maya-Repressor group </h3> | ||
+ | <p align="justify"> So we haven't been writing in the log for the last days as we have been really busy working in the lab and writing on the wiki. But after having realized that the Antiterminatorgroup still writes the log, I decided to write a little update.<br> | ||
+ | |||
+ | First of all we sent some stuff in for sequencing to find out whether we have mutations, as we thought we had. We got the results yesterday, and we found out that pIGR01, pIGR02, pIGR03, pIGR04 are not mutated. So the measurements we did on the biolector with these strains can indeed be trusted.<br> | ||
+ | |||
+ | Finally we had success in verifying pIGR11 meaning that the antirepressor antO is ready for submission.<br> | ||
+ | |||
+ | We also did a new round of ligation and transformation to get the pIGR05, pIGR06 and pIGR12 that we still haven't been able to verify. We changed the backbone in the pIGR05 and pIGR06 plasmids to pSB3C5, and this seemed to be a good idea because this time we got colonies that we could actually verify by PCR!!!!! :-) This means that we can prepare another biolector run, this time having all the planned constructs. But first we need to transform pIGR05 into a strain containing pIGR03, and pIGR06 into a strain with pIGR04. <br> | ||
+ | We haven't been able to verify pIGR12, so we will do another attempt tomorrow.<br> | ||
+ | |||
+ | We also did another experiment with Salmonella, but unfortunately this failed. We transformed pIGR03 and pIGR04 into Salmonella strains containing the antirepressors under the control of a pBAD promoter. Cultures were launched from the transformed colonies, and after having reached an OD of 2, some culture was transferred to LB+arabinose. The arabinose should induce the pBAD promoter causing expression of the antirepressor, again causing induction of the prophages, and de-repression of the repressor in the pIGR03/pIGR04 constructs which would finally result in GFP detection. We did indeed see lysis of the cells, but unfortunately no GFP expression could be measured when using the fluorometer. This result indicates that our plasmids produces too much repressor for the antirepressor to de-repress. <br> | ||
+ | |||
+ | Lastly, we registered all our biobricks in the partsregistry, and sent them all to the iGEM headquarter.<br></p> | ||
+ | |||
+ | <h3> 21-10-2010 - Patrick - Antiterminator group </h3> | ||
+ | <p align="justify"> Seemed like some of the cultures neither grew in the O/N cultures nor on the re-streaked plates, so new colonies were picked in order to have the 24 needed cultures for BioLector measurements.<br> | ||
+ | |||
+ | Once these had grown to what seemed to be exponential phase, OD was measured using Nanodrop and amounts of cultures needed for BioLector were calculated. | ||
+ | This followed by aliquoting the calculated amounts of the cultures (which apart from the new cultures, were in stationary phase) into fresh LB media in order to let them grow from ~ exponential phase and measured using BioLector; each culture was ran in duplicates.<br> | ||
+ | |||
+ | After the BioLector was started, we planned out the next set of measurements to run tomorrow which would be of SPL+RFP, J23100+RFP, J23101+RFP and J23116+RFP. O/N cultures were started of these combinations and will be ready for tomorrow's next BioLector run; the chosen colonies were also re-streaked for future reference.<br></p> | ||
+ | |||
+ | <h3>20-10-2010 - Patrick - Antiterminator group</h3> | ||
+ | <p align="justify"> The transformations that were re-done using the old batch of electrocompetent DH5-alpha cells turned out to have worked quite well, the negative ligation control plate had very few colonies whereas the plates containing the transformants had significantly more colonies, so very little background noise in our transformants. | ||
+ | The transformations that were done with XL1-blue had tiny colonies on them, so we need to let them grow longer in the incubator before we can make any conclusions on them.<br> | ||
+ | |||
+ | The remainder of the transformation cultures that were used to innoculate fresh LB media were measured using FACS, though as there were difficulties calibrating that spaceship and the uncertainty of FP references, data was obtained but there is bigger certainty that the BioLector measurements using single colonies will give more precise results.<br> | ||
+ | |||
+ | The plates containing colonies from EXII (reference - 19-10-2010) were used to make O/N cultures for BioLector measurements, these colonies were also restreaked for future use. <br> | ||
+ | BioLector measurements are set to take place tomorrow (21-10-2010).<br> | ||
+ | |||
+ | All parts to be sent to iGEM are now ready. <br></p> | ||
+ | |||
+ | <h3>19-10-2010 - Patrick - Antiterminator group</h3> | ||
+ | <p align="justify">Seeming as the transformants were first plated at 21:00 last night, couldn't make any conclusions after having looked at the plates in the morning; these will be left until the evening and checked again.<br> | ||
+ | As the newest batch of competent cells have some funky contamination, we re-did the transformations from yesterday using our oldest batch, although these are not extremely competent.<br> | ||
+ | Giving this a second thought, the ligations were remade from scratch again, using more DNA content, adding more ligations as well now that J23101 and more of I13507 were digested and ready for ligations.<br> | ||
+ | For these new ligations, a lab technician from another lab was kind enough to give us some XL1-blue electrocompetent cells which as we were told, were awesomely competent! :D<br> | ||
+ | These actually being alot more efficient when wanting to induce high copy number "mode" in pSB2K3 with IPTG as this strain contains lacIq as apposed to DH5-alpha which only contains lacI. <br> | ||
+ | Cultures have been prepared for FACS measurements for tomorrow.<br></p> | ||
+ | |||
+ | <h3> 18-10-2010 - Patrick - Antiterminator group </h3> | ||
+ | <p align="justify">pAT12-pAT16 were digested, cleaned up and run on a gel, they seemed good and were ready to be ligated.<br> | ||
+ | SPL was ligated with combinations between pAT12-pAT16 into pSB2K3; J23100 and J23116 promoters were also ligated with pAT15 into pSB2K3 as references for measuring with SPL.<br> | ||
+ | Once the above mentioned ligations were complete (x10) they along with J23100, J23116 and J23101 were transformed into DH5-alpha cells and then plated in amounts of 20ul, 100ul and 200ul. <br> | ||
+ | Hopefully the plates will give some good results tomorrow.<br></p> | ||
+ | |||
+ | |||
+ | <h3>18-10-2010 Repressor group Annemi, Lisa and Maya</h3> | ||
+ | <p align="justify">Ran a gel of the verification PCR Lisa did yesterday. Unfortunately the bands were nowhere to be seen.<br> | ||
+ | Did a PCR of the pIGR12 construct (Z2). Looks like we might have an insert in some of them. However in the lanes where our own primerF was used, no bands were visible. <br> | ||
+ | Wrote some descriptions of our BB's GR1, GR2 and Z1 and got it approved by Seb. So we should be ready to send those within the next few days.<br> | ||
+ | Sent the minipreps to sequencing and are now very excited to get the results. <br> | ||
+ | |||
+ | Started O/Ns of the minipreps that were sent for sequencing so we have backups. <br> | ||
+ | |||
+ | Thomas was very kind to do a verification PCR on our pIGR05 and pIGR06 constructs.<br></p> | ||
+ | |||
+ | <h3>17-10-2010 Juliet and Patrick- Antiterminator group</h3> | ||
+ | <p align="justify">I (Juliet) learned what not to do in the lab today :P but then Patrick and I made a new gel and ran a gel of the (50X) re-verification PCRs that Thomas made last night. We found that most of them were successful so we were able to proceed and make duplicates of PCRs of pAT12-pAT16. <br> | ||
+ | A gel was ran of the PCR's and their clean ups and turned out good, they are ready to be digested, ligated and transformed tomorrow. <br> | ||
+ | |||
+ | Parts to be sent to iGEM HQ have also been registered in the parts registry.<br></p> | ||
+ | |||
+ | <h3>16-10-2010 - Thomas - Antiterminator group</h3> | ||
+ | |||
+ | <p align="justify">Anastasiya and I did minipreps on the 30 overnight cultures that were started yesterday. We ran the minipreps on a gel and chose 25 plasmids to run verification PCRs on (so we only had to use 2 machines, and not 3). The results from the 50 PCRs were unfortunately inconclusive, so I redid them. I let them run in the machines overnight, so they are ready to be run on a gel tomorrow (amazing how 9-10 hours of work can be described with just 4 lines!).<br></p> | ||
+ | |||
+ | <h3>16-10-2010 Repressor group Annemi</h3> | ||
+ | |||
+ | <p align="justify">Ran a gel of the varification PCR products Lisa did yesterday. Some bands around 1200 bp and over 3 kb are slightly visible, however they don't look like PCR products. Lisa will redo the PCR tomorrow. <br> | ||
+ | |||
+ | Did a miniprep of the c-colonies 1-13 (except 7 which showed very little growth). Hopefully the minipreps c1-c6 will contain pIGR05 (pBADZ1, RFP), c6-c10 will contain pIGR06 (pBADZ2, RFP) and c11-c13 will contain RFP. <br> | ||
+ | |||
+ | Ran the minipreps on a gel. c11 looks gives a very weak band and no bands are visible in the lane with c13. <br></p> | ||
+ | |||
+ | <h3>15-10-2010 - Thomas - Antiterminator group</h3> | ||
+ | |||
+ | <p align="justify">Juliet and I did a PCR on pAT15 with primers IG201 and IG202, cleaned it up and ran it on a gel to reconfirm that the insert was correct. It was, so we started a digestion of the PCR product using X and P. We cleaned up the digestion and ran it on a gel to see the concentration. pAT15 is now ready to be ligated to the SPL! :). We also made O/N cultures of pAT12-16 (6 of each, 30 in total).<br> | ||
+ | |||
+ | After the digestion, Manos was ready to help Maya run her samples in the Biolector. Juliet and I helped her set it up, which took alot longer that expected since you have to measure the OD of each sample with the Nanodrop! With Manos' guidance, we loaded their 16 samples in the 48 wells (we did triplicates) and started the measurements.<br></p> | ||
+ | |||
+ | |||
+ | <h3>15-10-2010 Repressor group</h3> | ||
+ | |||
+ | <p align="justify">Verification PCRs were done. First batch were for verifying some old constructs of the biobricks that we're submitting. But as usual, the PCR failed. Maybe I shouldnt do 40 pcrs at a time (Lisa). | ||
+ | Next batch was to verify some newer construcst of BBs as well as a construct with pBADZ2 (pIGR06). Gel needs to be run tomorrow. | ||
+ | Also tried to make a table of all of the restreaks that we have, to get an overview, and we updated the other table of our constructs with which primers and melting temp you should use for verification. <br></p> | ||
+ | |||
+ | |||
+ | <h3>14-10-2010 - Thomas - Antiterminator group</h3> | ||
+ | |||
+ | <p align="justify">Anastasiya did minipreps of the O/N cultures of pAT13 and pAT15. Meanwhile I did PCR cleanups of the pSB3C5 and pSB3T5 backbone plasmid PCRs that Patrick did yesterday. I then did digestions of pSB3C5, pSB3T5 as well as J23100 and J23116, the two BioBrick promoters we plan to use as references in our measurements. After the minipreps were done, we ran verification PCRs on both plasmids and saw that only pAT15 had the correct insert.<br> | ||
+ | |||
+ | The ligations of pAT12-16 that were done yesterday seemed to have worked this time! Lisa and I restreaked six colonies of each construct, while Patrick did restreaks of the SPL + GFP construct, that also seemed to have worked.<br> | ||
+ | |||
+ | <b>NOTE:</b> It seems the newest batch of competent cells has been contaminated with some unknown E.coli strain that is also Amp resistant. This sucks alot if you are transforming plasmids with only Amp resistance. Sebastien says we just have to deal with it, since it's too late to waste time making a new batch (unless someone has nothing to do). Luckily the unknown E. coli strain seems to grow ALOT faster than DH5alpha, the "bad" colonies are giant compared to the "right" ones, so just avoid those when doing restreaks after a transformation.<br></p> | ||
+ | |||
+ | |||
+ | <h3>13-10-2010 - Patrick - Antiterminator group</h3> | ||
+ | |||
+ | <p align="justify">A gel was run of pcr cleaned up products: pAT02, pAT08, J23100 and J23116, these turned out good and are ready to be digested.<br> | ||
+ | |||
+ | As the transformed products that were re-plated yesterday didn't turn out to give any promising results, the ligations were remade of pAT12-pAT16. This time all new digestions seemed good and newly made competent cells were used as well. A ligation was made as well of SPL + GFP(+RBS) into pSB4A5, this merely to see the variation in GFP expression amoungst the colonies. The ligations were transformed and left to recover for 2 hours as apposed to the usual one hour, and then plated afterwards.<br> | ||
+ | |||
+ | Hopefully these new ligations work and it was merely a digestion problem before and nothing to do with the usage of pSB2K3 as the backbone nor resistance expression. <br></p> | ||
+ | |||
+ | <h3> 12-10-2010 Maya Repressor group </h3> | ||
+ | <p align="justify"> Restreaks of pIGR01 and pIGR07 (isnt it pIGR02? lisa 13-10) looked liked the previous restreaks. The colonies that were really green, were still really green.<br> | ||
+ | |||
+ | I made ligations of pIGR07 and pIGR08, and when I transformed I included that ligation mixture made the 06-10-10 containing pBADz1/z2 + RFP.<br> | ||
+ | |||
+ | Then I spend some time talking to Sebastien about sequencing. I will call the company tomorrow and ask what we need to do.<br> | ||
+ | |||
+ | I also talked to Jacobo about using the biolector Friday, and he will just make sure that he is not using it.<br> </p> | ||
+ | |||
+ | <h3> 12-10-2010 Patrick Anti-terminator group </h3> | ||
+ | <p align="justify"> Our constructs pAT12-pAT16 didn't seem to work, first reason could be cause of the pSB2K3 plasmid used, perhaps the cells were not left long enough to recover and hence express kanamycin resistance. Another reason could be the digestions made of pAT09-pAT11, as it seems the restriction enzymes were not given enough time, the gel illustrated that ~ half of each product was digested whilst the other half was not.<br> | ||
+ | |||
+ | Bottom line is, the transformed products were re-plated today in case they needed more time for resistance expression; all the products needed for the pAT12-pAT16 constructs were pcr'd and digested and ready for new ligations of pAT12-pAT16 if that is the case.<br> | ||
+ | |||
+ | Tomorrow a test will be made with the SPL, which will be ligated with GFP(+RBS) into pSB4A5.<br> </p> | ||
+ | |||
+ | <h3> 11-10-2010 Maya, Lisa and Annemi </h3> | ||
+ | <p align="justify"> Another day in hell... | ||
+ | Our restreaks with pBADz1/z2 and RFP don't seem to work. They don't grow up on glucose minimal media, and definitely not on ara+IPTG either. When looking at the original transformation plates it can also be seen that the colonies have different sizes indicating accumulation of mutations. This could be because the RFP or the antirepressor are toxic to e.coli, or because of something else. Anyways, we decided to transform the ligation mixture again, and this time plating on LB+Kan so that we don't induce RFP and antirepressor.<br> | ||
+ | |||
+ | RFP and GFP PCR products were purified, digested, purified again and run on a gel. They are ready for a ligation tomorrow.<br> | ||
+ | |||
+ | We also restreaked our pIGR01 and pIGR02 constructs to see whether the very green colonies will stay green meaning that in some way they are stable, or whether they will become white meaning that there is a pressure for accumulations of mutations in order to get rid of GFP.<br></p> | ||
+ | <h3> 11-10-2010 Anastasiya and Patrick Anti-terminator group </h3> | ||
+ | <p align="justify"> Started off the day by running digestions made yesterday (pAT09, pAT10, pAT11) on a gel, these were then pcr cleaned up, and then ran on a gel again. | ||
+ | On the gel we could see that the products were half digested (half were digested, other half not), thus we repeated the digestions of pAT09, pAT10 and pAT11.<br> | ||
+ | |||
+ | Using the digestions that were purified, we started the new ligation series of pAT12, pAT13, pAT14, pAT15 and pAT16, which are the 2nd final constructs before adding the SPL's.<br> | ||
+ | These were then tranformed and plated.<br> | ||
+ | |||
+ | Digestions were also made of SPL (E+S) and GFP+RBS (X+P) which will be ligated into pSB4A5 (E+P).<br> | ||
+ | |||
+ | Note: pcr clean ups of pAT09, pAT10 and pAT11 were all used up, if more needed of these products, new pcr's should be initiated.<br></p> | ||
+ | |||
+ | <h3> 10-10-10 Maya Repressor group </h3> | ||
+ | <p align="justify"> I made O/N cultures of the restreaks from 09-10-10. The restreaks are from the transformations made 06-10-10. There are no O/N of constructs containing pBADz1/pBADz2 as these grow much slower and were therefore not ready. <br></p> | ||
+ | |||
+ | <h3> 08-10-2010 Maya P2 lab </h3> | ||
+ | <p align="justify"> 100 ul of the O/N cultures originating from pIGR03 and pIGR04 were mixed with 3 ml of top agar and plated on LB plates with Amp. On top of the agar I added a small disc with 5 ul of mitomycin and a disc with 5 ul of water as a control. Ideally mitomycin should induce phage induction and thereby initiate expression of the antirepressor. The antirepressor should then de-repress the repressor allowing expression of GFP.<br></p> | ||
+ | |||
<h3> 07-10-2010 </h3> | <h3> 07-10-2010 </h3> | ||
<p align="justify"> Did transformations of the ligations made yesterday and plated these out on the right antibiotic plates. pBADZ1/2 were plated on the four different plates described yesterday. Hopefully we will see red colonies tomorrow.<br> | <p align="justify"> Did transformations of the ligations made yesterday and plated these out on the right antibiotic plates. pBADZ1/2 were plated on the four different plates described yesterday. Hopefully we will see red colonies tomorrow.<br> | ||
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<p align="justify">Digestions were made today of nutR and nutR+terminator both with restriction sites of XbaI and PstI; these will be used tomorrow for ligations of constructs pAT08 and pAT11, respectively.<br> | <p align="justify">Digestions were made today of nutR and nutR+terminator both with restriction sites of XbaI and PstI; these will be used tomorrow for ligations of constructs pAT08 and pAT11, respectively.<br> | ||
- | Mini preps of Mg03, Mg03+1C3, N+1C3, nutR+1C3 as well as puc19(one of Sebastien's high copy number plasmids) were made today, a few made in parallel while Sebastien did them as well, intention of this was to test whether mini prep skills were faulty or whether | + | Mini preps of Mg03, Mg03+1C3, N+1C3, nutR+1C3 as well as puc19(one of Sebastien's high copy number plasmids) were made today, a few made in parallel while Sebastien did them as well, intention of this was to test whether mini prep skills were faulty or whether our plasmids are simply in low concentration.<br> |
The restreaked plates containing our constructs of pAT02, pAT06 and pAT07 were used for innoculation of overnight cultures; these will be mini-preped tomorrow.<br> | The restreaked plates containing our constructs of pAT02, pAT06 and pAT07 were used for innoculation of overnight cultures; these will be mini-preped tomorrow.<br> |
Latest revision as of 16:13, 27 October 2010
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October23-10-2010-Maya-Repressor group Yesterday Sebastien transformed pIGR06 into a Salmonella strain to test whether the antirepressor works. Today I induced the pBAD promoter, which is infront of the antirepressor, by adding arabinose. After one hour I could see that the cells carrying the antirepressor-plasmid (pIGR06) lysed. This means that the antirepressor works:-) 22-10-2010-Maya-Repressor group So we haven't been writing in the log for the last days as we have been really busy working in the lab and writing on the wiki. But after having realized that the Antiterminatorgroup still writes the log, I decided to write a little update. 21-10-2010 - Patrick - Antiterminator group Seemed like some of the cultures neither grew in the O/N cultures nor on the re-streaked plates, so new colonies were picked in order to have the 24 needed cultures for BioLector measurements. 20-10-2010 - Patrick - Antiterminator group The transformations that were re-done using the old batch of electrocompetent DH5-alpha cells turned out to have worked quite well, the negative ligation control plate had very few colonies whereas the plates containing the transformants had significantly more colonies, so very little background noise in our transformants.
The transformations that were done with XL1-blue had tiny colonies on them, so we need to let them grow longer in the incubator before we can make any conclusions on them. 19-10-2010 - Patrick - Antiterminator groupSeeming as the transformants were first plated at 21:00 last night, couldn't make any conclusions after having looked at the plates in the morning; these will be left until the evening and checked again. 18-10-2010 - Patrick - Antiterminator grouppAT12-pAT16 were digested, cleaned up and run on a gel, they seemed good and were ready to be ligated. 18-10-2010 Repressor group Annemi, Lisa and MayaRan a gel of the verification PCR Lisa did yesterday. Unfortunately the bands were nowhere to be seen. 17-10-2010 Juliet and Patrick- Antiterminator groupI (Juliet) learned what not to do in the lab today :P but then Patrick and I made a new gel and ran a gel of the (50X) re-verification PCRs that Thomas made last night. We found that most of them were successful so we were able to proceed and make duplicates of PCRs of pAT12-pAT16. 16-10-2010 - Thomas - Antiterminator groupAnastasiya and I did minipreps on the 30 overnight cultures that were started yesterday. We ran the minipreps on a gel and chose 25 plasmids to run verification PCRs on (so we only had to use 2 machines, and not 3). The results from the 50 PCRs were unfortunately inconclusive, so I redid them. I let them run in the machines overnight, so they are ready to be run on a gel tomorrow (amazing how 9-10 hours of work can be described with just 4 lines!). 16-10-2010 Repressor group AnnemiRan a gel of the varification PCR products Lisa did yesterday. Some bands around 1200 bp and over 3 kb are slightly visible, however they don't look like PCR products. Lisa will redo the PCR tomorrow. 15-10-2010 - Thomas - Antiterminator groupJuliet and I did a PCR on pAT15 with primers IG201 and IG202, cleaned it up and ran it on a gel to reconfirm that the insert was correct. It was, so we started a digestion of the PCR product using X and P. We cleaned up the digestion and ran it on a gel to see the concentration. pAT15 is now ready to be ligated to the SPL! :). We also made O/N cultures of pAT12-16 (6 of each, 30 in total). 15-10-2010 Repressor groupVerification PCRs were done. First batch were for verifying some old constructs of the biobricks that we're submitting. But as usual, the PCR failed. Maybe I shouldnt do 40 pcrs at a time (Lisa).
Next batch was to verify some newer construcst of BBs as well as a construct with pBADZ2 (pIGR06). Gel needs to be run tomorrow.
Also tried to make a table of all of the restreaks that we have, to get an overview, and we updated the other table of our constructs with which primers and melting temp you should use for verification. 14-10-2010 - Thomas - Antiterminator groupAnastasiya did minipreps of the O/N cultures of pAT13 and pAT15. Meanwhile I did PCR cleanups of the pSB3C5 and pSB3T5 backbone plasmid PCRs that Patrick did yesterday. I then did digestions of pSB3C5, pSB3T5 as well as J23100 and J23116, the two BioBrick promoters we plan to use as references in our measurements. After the minipreps were done, we ran verification PCRs on both plasmids and saw that only pAT15 had the correct insert. 13-10-2010 - Patrick - Antiterminator groupA gel was run of pcr cleaned up products: pAT02, pAT08, J23100 and J23116, these turned out good and are ready to be digested. 12-10-2010 Maya Repressor group Restreaks of pIGR01 and pIGR07 (isnt it pIGR02? lisa 13-10) looked liked the previous restreaks. The colonies that were really green, were still really green. 12-10-2010 Patrick Anti-terminator group Our constructs pAT12-pAT16 didn't seem to work, first reason could be cause of the pSB2K3 plasmid used, perhaps the cells were not left long enough to recover and hence express kanamycin resistance. Another reason could be the digestions made of pAT09-pAT11, as it seems the restriction enzymes were not given enough time, the gel illustrated that ~ half of each product was digested whilst the other half was not. 11-10-2010 Maya, Lisa and Annemi Another day in hell...
Our restreaks with pBADz1/z2 and RFP don't seem to work. They don't grow up on glucose minimal media, and definitely not on ara+IPTG either. When looking at the original transformation plates it can also be seen that the colonies have different sizes indicating accumulation of mutations. This could be because the RFP or the antirepressor are toxic to e.coli, or because of something else. Anyways, we decided to transform the ligation mixture again, and this time plating on LB+Kan so that we don't induce RFP and antirepressor. 11-10-2010 Anastasiya and Patrick Anti-terminator group Started off the day by running digestions made yesterday (pAT09, pAT10, pAT11) on a gel, these were then pcr cleaned up, and then ran on a gel again.
On the gel we could see that the products were half digested (half were digested, other half not), thus we repeated the digestions of pAT09, pAT10 and pAT11. 10-10-10 Maya Repressor group I made O/N cultures of the restreaks from 09-10-10. The restreaks are from the transformations made 06-10-10. There are no O/N of constructs containing pBADz1/pBADz2 as these grow much slower and were therefore not ready. 08-10-2010 Maya P2 lab 100 ul of the O/N cultures originating from pIGR03 and pIGR04 were mixed with 3 ml of top agar and plated on LB plates with Amp. On top of the agar I added a small disc with 5 ul of mitomycin and a disc with 5 ul of water as a control. Ideally mitomycin should induce phage induction and thereby initiate expression of the antirepressor. The antirepressor should then de-repress the repressor allowing expression of GFP. 07-10-2010 Did transformations of the ligations made yesterday and plated these out on the right antibiotic plates. pBADZ1/2 were plated on the four different plates described yesterday. Hopefully we will see red colonies tomorrow. 07-10-2010 Maya - Still Depressor group Yesterday I just did some restreaks of the transformations I made 05-10-2010. Today I had a look at these, and it was very obvious that the pIGR01 (G1+GFP) construct in the 421 (WT) strain looked really sick. This is most likely because the pR promoter is too strong and we get too much GFP expression. We thought that the repressor, which is naturally in the salmonella, would repress the pR promoter, but this was not the case.
B expressed 30% less GFP (says Flemming). We would have expected the repressor from the Salmonella prophages to shut down expression from the pR promoter more efficiently. D hardly expressed any GFP. This was both good and bad. Good because it indicates that we have a correct plasmid since GFP is present. Bad because the repressor in the GR1 construct should shut down expression 100%. I made O/N of the restreaks from yesterday. 06-10-2010 - Greg and Juliet - WikiGreg worked on some of the figures and changed the layout for our poster. I worked on the wiki, changing the layout ~ essentially beautifying it and so the plan is to read through the content and figure out what needs to be edited and added and who should do it (even if it's me) ;) which means that I will probably be bossy and demand things from people, so be prepared! ;) 06-10-2010 - Patrick - Anti-Terminator group The SPL PCR product was ran on a gel, and looked quite good having a band size just around 1kb, its actual size being 941bp, so thats pretty good, PCR clean up was then performed on it. 05-10-2010 - Patrick - Anti-Depressor Group: The Terminators!!So it seems like our competing team isn't doing too well, so we will try helping them out tomorrow if they need it. :)
The template used in order to obtain the chloramphenicol cassette was pKD3, which was kindly supplied by Sebastien. Note: I made the PCR using the Phusion enzyme, running a normal PCR program, not the one we've always been running which contains ramp TD settings; I did this PCR on the old PCR machine in the 2nd last lab down the hallway.
05-10-2010 Maya DEPRESSOR groupSo today I did a lot of crying... We really need some good results soon!!
All plasmids are from the 02-10-10 I plated 100 ul on Amp plates. The colonies need to be re-streaked tomorrow, and the day after tomorrow, the restreaked colonies can be plated on plates containing phage inducing compounds (this will induce expression of the antirepressor). What we hope to see from this experiment is whether the G1/G2 construct will stop expression of GFP when transformed into the 421 strain, as this strain produces the repressor which will act on the pR promoter. We also expect the antirepressor to de-repres the repressor in the GR1/GR2 construct, thereby starting expression of GFP. The 413 strain is used as a control. 05-10-2010 Annemi Depressor group!!!Did a PCR of the mini-preps from October 2nd and 4th (see labbook for further detail) but this time diluted 100 fold in water. 05-10-2010 Juliet and GregWiki: layout improvements in project description. Refactoring of text in project desc. Updates for blog, front page and team. 04-10-2010 Patrick and AnastasiyaWe have done PCR clean up of the PCR products from 03.10 (pAT01-1, pAT01-2, pAT08-1) and run them on the gel to verify their sizes. Glycerol stock solutions of pAT01-1 and pAT08-1 have been prepared. Then we have done restrictions of pAT08 (E, S) and pSB2K3 (E, P). Ligation products from 03.10 (pAT09, pAT10, pAT11) have been transformed.
3 & 4-10-2010 Repressor group Lisawe did PCR on minipreps - and there are nothing going on in the PCR. What are we doing wrong? 04-10-2010 WIKI References (Malthe)Hi team I have with support from Juliet and Greg, tried to set up a footnote or reference system on our wiki, igem have not intalled the application needed and thus the references have to be typed in with text. se example in the "Project" page. 04-10-2010 - SDU DTU iGEM conference - MaltheUpdate: We have booked the seminar room here in 301, to avoid problems with keys ect. Regarding food i talked to Lene Krøl (info below). we decided that either we get a "factura" and give them and they pay. when this is not possible, when shopping in a supermarket, we pay and get the money refunded, save the receipt. 03-10-2010 - Thomas - Antiterminator groupJuliet and I were in the lab today the group. We ran a gel of the 30 verification PCRs that were done yesterday, as well as the four restriction digests. The verification PCRs showed that pATN and pAT08 were both successfully ligated and that the pAT11 ligation failed. We're unsure about the pAT01 ligation, there were strong bands for all four minipreps done, but one of the inserts was larger than the other three. The one that was larger was also the one we thought was closest to the expected size. We ran three PCRs, two of pAT01 (to further verify it) and one of pAT08 so it will be ready for restriction tomorrow. 02-10-2010 Anastasiya & Patrick Anti-terminator groupRe-did the digestions on pAT02, pAT04, pAT06 and pAT07 that Thomas managed to kill last night.. :p They were ran on a gel and seem to be good, PCR clean ups were made on them and they need to be ran on a gel again to determine the dna concentration, so this is one of the tasks to do for tomorrow.
Freeze solutions were made of pAT02(L1-2), pAT06(L2-4), pAT07(L4-4) and placed into our strain bank in the -80C freezer. 02-10-2010 Repressor group AnnemiMade minipreps of the overnight cultures from yesterday. Made with 4mL culture. They are stored in the freezer in a blue thingy. Should be easy to find.
Ran a gel of the minipreps. 01-10-2010 - Thomas - Antiterminator groupRan a gel of PCR products of pAT02, 04, 06 and 07 (from 30-09) and then a PCR clean up and another gel of that. Both gels looked good, each band was the expected size. The purified PCR products were then digested with X and P. 01-10-2010 Repressor group Maya and LisaThe restriction products from yesterday (G1, G2 and RFP), and the PCR products RFP and GFP were purified and run on a gel. Everthing looked good, and this was the first time that we could actually see G1 and G2 on the gel after restriction. This was probably because two pcr products were pooled in one clean-up, and because the restriction was done in only 50 ul total volume rather than 100 ul.
We made a PCR of the pSB4A5 and the pSB1C3 backbones. These were purified, but the purified products were not run on a gel as we didn’t have the time. Finally, O/N cultures of the restreaks from yesterday were done. 23 in total. Three of the restreaks containing pSB4A5 and GFP were red, and as they are not supposed to be that, these were of course not included in the O/N’s. Tomorrow minipreps of the O/N’s and a PCR can be done, and then we will hopefully know whether we have some constructs that are ready for measurements. 01-10-2010 Dry Lab - Anja
Septermber30-09-2010 Dry Lab - Anjanice that the dry lab people also are allowed to write in the Lab blog now :-)
30-09-2010 Anastasiya Antiterminator groupThomas and I have done 2 PCR verifications on each of the MiniPreps prepared on 29.09, corresponding to ligation products L1-L5 namely of pATO2, pAT06 and pAT07. We run 40 PCR reactions in total. (For further information see our lab book) Then we run them on gel to verify their sizes and see if they worked. It seems like all of them have worked except from pAT06, but likely we have run it twise and at least one of them worked.
30-09-2010 Maya Repressor groupAnnemi's 40 PCR reactions from yesterday didn't give any result, meaning that we still haven't succeeded in ligating our biobricks into pSB1C3. We will put this on pause for now and concentrate on ligating our biobricks into pSB4A5/pSB2K3 with GFP/RFP. 29-09-2010 Greg Repressor groupGot in touch with students using the BioLector (Manos and Jacopo). Made a tentative booking for weekend 9-10.10.10 (Friday 8th also possible). Jacopo will explain how to use the equipment a few days before we run the plates. Recommendation is to measure OD of a culture grown outside of Biolector (but in the same medium) to have an estimate of when best to treat with arabinose (this applies to the antirepressor system). Should treat during exponential phase. Also it's important to prepare the plate under the hood, to avoid contamination. 29-09-2010 Annemi Repressor groupMade ligations of the following:
Transformed the ligations in electrocompetent cells DH5α Plated the transformants on plates (20 and 200 µL) Ran a PCR of the minipreps done yesterday using IG202 as the reverse primer for all (40!!!) reactions. IGR01 used as forward on miniprep 1-5 + 11-15. IGR04 used as forward on miniprep 6-10 + 16-20. IG201 used as forward on 1-20. Further detail on the programs can be seen in the labbook. Very busy day in the lab and hopefully we will get some results:) 29-09-2010 Thomas & Patrick Antiterminator groupStarted off the day by making ligations of our constructs: pAT01, pAT08 and pAT11. These were then transformed and plated; they will be ready for restreaking tomorrow and innoculation of overnight cultures on the subsequent day. Mini-preps were made from the over-night cultures containing our constructs pAT02, pAT06 and pAT07; these will be PCR verified tomorrow. 28-09-2010 Patrick Antiterminator groupDigestions were made today of nutR and nutR+terminator both with restriction sites of XbaI and PstI; these will be used tomorrow for ligations of constructs pAT08 and pAT11, respectively. 28-09-2010 Greg Repressor groupMoved last year's layout to the home page. The links have been updated and should work (let me know if they don't). 28-09-2010 Annemi Repressor groupToday the PCR of G1, G2, GR1, GR2, BADZ1 and BADZ2 was redone and it looks good:) 27-09-2010 Maya Repressor groupThe PCRs I made the 24-09-2010 were ran on a gel i the weekend and no bands appeared:-( Maybe something is really wrong, or maybe I'm just really bad at making PCRs. Sebastien had a look at the gel picture with the purified plasmids that I used as templates and thinks that they look weird. He thinks the concentration is way lower than normally, and he also thinks they look like cut plasmids. So I'm not sure whether we should attempt a new miniprep or whether we should make a new PCR on the miniprep I did, or start all over... We did after all have a lot of background in this ligation, so maybe its a good idea to start over. Sebstien also mentioned that it could be a problem to try to clone the gifsy repressors into pSB1C3 which is a high copy number plamid, and as far as he understood it, the IGEM headquarter allows submission in other plasmids if you have an explanation for not using pSB1C3. So I guess we could just submit in pSB4A5. Anyways, we can talk about this tomorrow as I'll come in at 8 am. 27-09-2010 - Anastasiya & Patrick - Anti-terminator groupRestreaks were made of ligation plates of L1 to L5 that can be found in the lab book dated 23rd September 2010.
Over night culture media (already containing antibiotics) are ready and stored in the fridge, these will be used for the colonies obtained from the restreaks mentioned above. 25-09-2010 Repressor group MayaYesterday I was in the lab alone, but fortunately Patrick was kind enough to help me out a bit. I did minipreps of the 20 O/N (5 colonies from each transformation) that Annemi and I did yesterday. These minipreps hopefully contain our PCR products (G1, G2, GR1 and GR2) in the pSB1C3 backbone. After the miniprep I did 40 PCR reactions on the plamids. All plasmids were tested with two sets of primers - the VF1 and VR primers and also with our IGR01/IGR04 & VR primers. Today I'll go the lab and put the PCR products in the fridge, and if I have time I'll run them on a gel as well. 24-09-2010 - Thomas - Antiterminator groupThe transformations of our ligations from yesterday look really good! :). There are only about 8 colonies on the ligation control, and 20+ on the plates with the actual ligations. We restreaked 4 colonies of each of the 5 ligations and put them on the lab bench to let them grow over the weekend. On Monday we should start some overnight cultures of all 20 restreaks so we can miniprep and verify them on Tuesday. 23-09-2010 - Thomas - Antiterminator groupUnfortunately, I was in the lab alone today, due to half my group being on vacation. Since I had to prepare the presentation for the meeting with our supervisors and the 2009 team in the afternoon, not alot got done in the lab. I transformed the ligations that Patrick did yesterday, with Anja's help, and plated them. Anja ran a gel of the PCRs of the plasmids backbones that Patrick did yesterday and they all looked good. Anja also did a miniprep of the MG03 plasmid :). 23-09-2010 Maya Repressor groupToday we got the proof that the plasmids pSLD20 and pSLD22 have been mixed up during O/N or miniprep. This means that the plates we have in the fridge are correct, but that the plasmids are swapped in the glycerol stock. We haven't corrected the naming, but will do that tomorrow. 22-09-2010 Annemi Repressor groupColony PCR on transformations G1, G2, GR1, GR2. Same approach as Lisa did yesterday, however we marked the colonies this time:)
Did a PCR clean-up -> working box tubes with white stickers provided with: date, DNA, RE-info, 'cleanup' Next move: Run gel of the cleaned up restrictions. 22-09-2010 Maya Repressor groupWe still haven't figured out what happend to the plasmids pSLD20 and pSLD22, so we restreaked both the ones from the glycerol stock and the ones in the fridge. 22-09-2010 - Patrick - Terminator groupAnother long busy day with many items to take care of.
A digestion was also made on RBS-N with X+P, this needs to be purified via pcr clean up tomorrow (23/09/10). Once purified it can be used along with pBAD (E+S digested) and pSB4A5 (E+P digested) to construct pAT01 which should look like the following:
PCR duplicates were made today and will be ready tomorrow (23/09/10), the following plasmid backbones were amplified:
- These need to be verified tomorrow (23/09/10) on gel to make sure they were in fact amplified, followed by pcr clean up. 2 extra pcr duplicates should be made of the following:
Another over night culture was made of Mg03 as a mistake was made yesterday and the wrong anti-biotic was inserted. This needs to be plasmid purified tomorrow as well. Find to do list in lab book, same content will be present there as here. If you have any questions about this, gimme a call or find me in lab 201 tomorrow. Over and out. 21-09-2010-Lisa - Repressor groupA new PCR with pBAD, BADZ1 and BADZ2 turned out to be succesful, as Annemi wrote (using miniprep 1 as template) - although it seems that there is confusion about which plasmid is pSLD20 and which one is pSLD22. Sebastien says to trust the PCR products! and he might have an explanation for the mix up. Talk to him tomorrow. 21-09-2010 - Patrick - Terminator groupToday the lab work was ran almost parallel with good success with the repressor group, Lisa and I had a rather successful day.
To start off with, the PCR's in the morning.. WORKED!! Those were both from the repressor group and terminator group.
The second gel made contained the above mentioned digestions as well as Lisa's colony PCR's. From the gel its hard to evaluate the outcome of the digestions as they were made on pcr products, but non the less bands were visible for all 5 of the digestions run with matching bp sizes. The other 15 bands were repressor groups colony pcr's (both repressor and terminator groups have the gel pictures in their lab books). Over night cultures were made of the re-streaked ligation plates, tomorrow (22/09/2010) plasmid purifications need to be performed. Tomorrow ligations on pAT02, pAT06, and pAT07 need to be done. 21-09-2010 - Annemi Repressor groupA new attempt to amplify pBAD, pBADz1 and pBADz2 was made. The PCR was made exactly as Maya made it yesterday (see lab-book for further details). 20-09-2010 - Patrick and Anastasiya - Terminator groupSo today we've been doing a bit of work for both the terminator and repressor group.
Firstly we ran 2 pcr's on plasmid backbones (pSB1C3 and pSB2K3) which turned out successful on the gel, they were then purified via pcr clean up.
(Please take note here that the old pcr buffer was used, so I suggest from now on when running a pcr, use any buffer you think will work, but use the old buffer as a form of control with an extra pcr product, so that in case it doesn't work but the control does, the problem might be the buffer and not your pcr.) 20-09-2010 - Maya -Repressor groupThe PCR Lisa and I did Friday only worked for the pBAD promoter, not for the pBADAntO or pBADAntT. So today I redid the PCR using each primer set on both pSLD20 and 22 just in case Sebastien messed up the labeling of the plasmids. I also restreaked the pSLD 20 and 22 on plates with CAM and KAN to verify whether Sebastien did indeed mess up labeling. Patrick will run the products on a gel, and place the photo on our desk today. If the PCR is still not working we should talk to sebastien about alternative ways of amplifying the products. 17 -09-2010 - Lisa and Maya - repressor groupGel of the purification of G1, G2, GR1 and GR2 looked good, we did ligations of these parts with the plasmid pSB1C3 - these ligations should be transformed monday (20-09-2010). 16-09-2010 - Maya and Annemi - repressor groupWe did a restriction on our PCR products (G1, G2, GR1 and GR2), and of the plasmid pSB1C3. The plasmid is going to be used for submission of the biobricks. The restrictions were purified using the PCR purification kit. The purified products still need to be run on a gel. If the gel looks good tomorrow, a ligation should be done. 16-09-2010 - Anja - repressor group
15/09/2010 - Terminator group - Thomas & PatrickToday we did digestions of N, NutR, MG03, pSB1C3. After PCR-cleanup the N and NutR digestions seemed to have worked but you can't see a difference from digested/non-digested as they are from pcr products. The MG03 digestion looks bad, but the dna concentration might have been too low. The pSB1C3 also had a low dna concentration. Tomorrow we will still attempt ligations and redo digestion of both MG03 and pSB1C3. We should also pcr more linear pSB1C3 plasmid backbone. 14-09-2010 Anja (Repressor group)Lab stuff:
There are different ways to get more supplies:
to repressor group: I finished the A3sized paper Maya started yesterday, so Maya maybe you can have a second look at it, feel free to add or change, of course :-) Plasmids: to repressor group With regard to our plasmid pSB4A5, pSB2K3 and others: I suggest that we make our own linearized plasmid, so we don´t have to worry whether the insert is cut out or not. This is done by using primers IG206 and IG207. These primers have been ordered by Thomas, so there is no time delay, when using this approach. For further information see parts registry help > protocols > linearized backbones. Please think about how we can purify our biobrick I_13507 from gel, to get rid of the plasmid, we don´t need. - we just do an ordinary BB transformation Wiki: Lisa started on reading articles and hasn´t decided which topic she wants to write about. I signed up for repressors in Juliets wiki sheet. 15. sep. 2010 AnnemiToday we have run PCR´s to amplify the promoter region and the repressor region. We used 2µL of Sebastiens Salmonella DNA number 143 as template.
(See the lab book for further detail on the procedure) 13-09-2010 Maya (repressor group)Today me and Anastasiya did O/N cultures of the biobricks that we transformed last week. Tomorrow we need to do a miniprep on all of these plasmids, and also prepare some glycerol stocks. We made double of the O/N so there should be enough if you want each group to have their own sets of purify plasmids. 080910 Maya and Annemi (Repressor group)We now have a strategy on how to do the labwork in the repressor group. We will need to construct six different plasmids:
August31-08-2010IGEM UPDATE: 31-08-2010 (copied to log) The Result of the Day, and what we talked about. BB REGISTRATION - REPRESSOR & ANTI-TERMINATOR
AGENDA - So far
management deadline 20-sept.
24-08-2010So the competent cells we made last week have been infected by phages!!! Oh no, this is really bad cuz it's difficult to get rid of phage contamination. Sebastien thinks that it might be a T1 phage. So we are preparing to make a new batch of competent cells. This will be done Friday. All the pipettes have been cleaned thoroughly to get rid of potential contamination. 20-08-2010 (Patrick , Malthe , Anja, Juliet and Maya)To make it easier for everyone to follow the project I'll try to give an update on what has been going on this week.
Social event: Free Funky jazz concert saturday Hezz brothers. http://kglteater.dk/Alle_forestillinger/DKTplus_10_11/Hess_is_more.aspx Looking forward to everyone is back:-) It really seems like we are on the right track now. Whats going on in the lab (12/08/10) (Annemi, Patrick)So if you have done your homework and read yesterdays log ;), you would have a better understanding and update of whats going on with the project.
Heres whats actually going on in the lab right now:
Lab work - follow up (11/08/10) (Lisa, Annemi, Thomas, Anja, Anastasiya & Patrick)As the log was supposed to be updated according to the successes based upon construction of a template plasmids containing the FP's, the reason why this never occured is because it never worked and a huge change in the project occured. JulyLab work (Patrick, Anastasiya and Anja) 06/07/10After last weeks succesful ligation of CAM and KAN resistance markers into plasmid pSLD3, we successfully constructed plasmids pSLD30 (which contains CAM) and pSLD31 (which contains KAN). All the steps and how we calculated the volumes needed of all the items for both restriction and ligation can be found in the lab book. Long story short, in order to have ample amounts of inserts, (FP's and resistance markers), we performed PCR's.. both de-novo amplifications of the inserts that weren't present as PCR products from Sebastien already, and re-amplications of the PCR products available from Sebastien. Once PCR was completed, we had ample amounts of all the FP's (yGFP, CFP, and CRFP) as well as resistance markers (CAM & KAN).
The next step was the ligation. Ligation (follow lab book protocol) pretty much doesn't need an explanation as it ligated plasmid with insert. The ligations were also checked on gel to make sure ligation actually occured. This was followed by transformation, were we used the method of electroporation to insert our newly constructed plasmids (pSLD30 + 31) into electrocompetent cells, incubate them at 37 degrees in recovery media for 2 hours and then plate them on the corresponding needed plates. These plates (9 in total) were left over night in the incubator (37C) to grow and have a party. In the lab book you can get an overview of what each of the these 9 plates contained, there were of course several controls as you might have guessed. The plates of most importance were the ones containing the transformations containing plasmids pSLD30 and pSLD31, thus from these plates one colony was used for a restreak on a new plate to have as a "stock" plate, as well as making over-night cultures. The over-night cultures, obviously having grown over-night were used to perform plasmid purification (follow protocol) in order to obtain pSLD30 and pSLD31, -80 freezing cultures of the strains were also made and registered in the "strain bank" excel file found in dropbox. So, from A to B, the steps were the following:
Have a look at the lab book in order to get a full detailed explanation of all of these steps and all the small details not mentioned here. Next step are the insertions of all the FP's (yGFP, CFP & CRFP) into pSLD30 and pSLD31, individually of course.. will make that tomorrow's log. Over and out (Patrick). JuneLab work (Thomas, Anja, Patrick and Maya) 25/06/10Today Thomas joined the lab:-) You can't spell funding without fun... (Annemi) - 25/06/10I had a look at some funding and where we should go from here.
Birthday and fun day at the lab? (Maya, Anja, and Patrick) - 24/06/10So today was yet another day in the lab, only difference being it was my birthday (Patrick). :D Progress (Maya, Anja, and Patrick) - 23/06/10So we started in the lab yesterday after having gotten all the needed information from Flemming concerning the FP's (fluorescence proteins). iGEM the last 2 weeks - 21/06/10So the last 2 weeks have been quite hectic and busy, and if you're wondering why there hasn't been an update its because alot of things keep coming up while working on the design. Maya, Anja, Malthe and Patrick's log - 08/06/10We have finished the step-wise construction of our system, and have begun on the in-silico model. Maya and Patrick's log - 07/06/10So today we have been working on the step-wise construction of our system, taking into account how to test each part along the way. We learned a lot about recombineering and the factors entailed in the process and have come up with the initial version of how we are going to construct the system.
We have also uploaded Sebastien's presentations from last week, and they can be found in the folder "Presentations from Sebastien" in the research group folder as well. So, from all the work today we are trying to make a scheme of phases / phase planning of the construction parts that need to be completed in a described order that will be uploaded possibly within this week. Captain's log 040610Maya, Thomas, Patrick, Lisa and Annemi have been working on a project description for Sebastien. The document 'project description' can be found in dropbox in the research group folder. From now on this document will be the only one describing the project, therefore you should edit in the document and not create a new one. We have decided that every time we are doing something iGEM related, that it should be posted in this document. Please write the date and your name at the beginning of your log. This will make it easier for all of us to keep track of what is going on in the group. We have tried to make a simple plan of what needs to be done before going to the lab:
Maya will start creating an illustration for the system during the weekend. Thomas will delete all irrelevant budgets from the dropbox. He will also send the project description to Sebastien. |