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CAROL
Ligation of promoter library and pCS26 and Transformation of plasmid in E. coli
- Following the overnight enzyme digestion (BamHI and XhoI) of the vector (pCS26) and promoter (created by the 32 different primers), the vector (pCS26) was treated with anarctic phosphatase for 30 minutes (see proper protocol in procedure page) and the products was ligated with 3 different methods:
1. NEB Quick Ligase for 5 minutes
2. Invitrogen T4 Ligase at 16oC overnight
3. Invitrogen T4 Ligase at room temperature (~21oC) for one week
- The Quick Ligated product was transformed into Top 10 cells and was grown on LB plates with Kan resistance for 16 hours.
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CHINMOYEE
Programing of Hill curve fitting Complete
Watched the Awesome Molecular biology video . Learned quite a bit about cells in our body . Set up Matlab so that when data is present the Hill Equation will automatically fit the data to a curve .
At the end of the Day we had a fire alarm.
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EMILY
DNA Sequencing & Wiki Updating
- Today I sent one of the colonies from my restriction digest yesterday down for sequencing. When these results come in, we will be able to see if the B0015 terminator has been successfully cloned into the J13002-LuxOD47E construct. If this is succesful, my circuit will be done! From here, I can use the parts that Kevin has been contructing with GFP to put my circuit in and test the functioning of my circuit.
- This afternoon I helped Mandy with editing more photos for the Wiki. I also looked about CedarLane Laboratories, our sponsor of the month, and wrote a short paragraph about them to include on our Wiki. I also sent an Ethics paper that Fahd sent me.
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FAHD
Marketing for July 17th 2009
Today, I concentrated my energies at marketing our iGEM project and looking at the ethical aspect of our project. Here is what I did today:
1) Attended Meeting
2) Did my ethics blog
3) Did not call and e-mail any companies because it was too late in the day
4) Talked to Nexen and told her that when she meets with her manager on monday, please tell him that any kind of donation would help because we are developing educational tools and our project has potential applications such as bioremediation.
5) Read Ethics papers
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IMAN
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JAMIE
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JEREMY
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KATIE
A Little Bit of Everything
The phosphatase treatment station is now set up to listen for the queue that all ingredients have been added and then moves the phosphatase tube to the water bath, which is also set to listen for the tube as it travels to the bath. Once just outside the water bath will lift the lid and the tube will go inside. At the moment, after this has been completed it just appears at its original position on the a lab bench, but I think I will make it travel back more slowly as phosphatase treatment is explained once I have time to write up some basic instructions.
The listen scripts are complete for restriction digest and the heating block and now all I need to do is incorporate them into the existing scripts within the objects. The test tubes will then have to be moved to the water bath, heating block and freezer (for insert), which should not be a problem since the phosphatase tube is already set up so the script will not be much different.
Basic instructions for construction and bacterial transformation have been completed, which I will still have to add to the touch_start event or have them beside the activity. The bacterial transformation quiz also had to be able to be reset at any time so each question for the quiz now has a reset button for a choice and when touched, it will not only reset any variables for the quiz, but reset the progress test tube to the original white/transparent colour
I was able to modify the notecard reader script so that it will check that the contents within two notecards are the same, which I think I will use in the sequencer as well as the construction tubes. The notecards can contain a series of bases that will determine if it is a promoter, rbs etc. And how it has been cut so I will not just be relying on checking for the proper name of the notecard, but what it contains. You can also add the information from two notecards together, but this will only be useful if I can determine a way to store the information in a notecard and give it to the individual. I do not know if it is possible to make a new notecard with a script or if there is only one empty notecard, if you put the information into it and give it to a user I do not know if the notecard in the objects inventory would remain empty, which is what I would want. I will be looking into this next week.
I also plan to prepare something for the blog video I have to do by Tuesday where I will display the progress that has been made in the lab as well as some of the scripts that are behind the functionality of the objects.
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KEVIN
1. Plasmid Isolation of B0034
I have isolated the plasmids from these overnight cultures, and the purity and concentration of them were measured using nanodrop. They were pure enough to move on with.
2. Construction of Pqrr4+B0034
Since our Luciferase did not turn out great, we turned our attention to GFP:LVA. But because the part with GFP:LVA does not contain RBS, I need to constrct Pqrr4+B0034 first. Pqrr4 was cut with SpeI+PstI and B0034 was cut with XbaI+PstI. Pqrr4 was then phosphotase treated, and the two were ligated together. The ligated product was finally transformed into TOP10 cells. Carol promised to take the plates out tomorrow.
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MANDY
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PATRICK
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PRIMA
Media Inquiries
After the marketing meeting, I contact Sembiosys, called up the Investor Relations Inquires lead, Abby Garfunkel and told her about our project. She asked me to mail her the sponsorship pkg so she could forward it to Dr. Moloney. I wrote an email to Dr. moloney restating our project goal, meeting and that I spoke to Abby. The rest of the marketing team checked over the email before I sent it out. Hopefully, he gets back to me soon or I’ll call Ms. Abby again on Tuesday.
I found a number for Jay Ingram but I couldn’t find any emails anywhere on the websites. However, I spoke to Dr. Jacob today and he said he knew Mr. Ingram and his wife and he’ll send me her email address and hopefully I can get a hold of him through her. I started writing the email that I’m going to send to Jay Ingram. Dr. Jacob wanted to know how we’re doing in marketing so I told him everything and about our marketing meeting this morning.
Oh and I sent Mandel Scientific an email asking for a pipet set and pipet tips. So next week, I have to follow-up with a WHOLE BUNCH OF companies (about 10 –pratically all the ones I’ve mentioned over the past 2 days). I also updated the iGEM marketing company list on gmail spreadsheet.
Finally, I just helped Jamie with plating after he transformed Cl lambda earlier today.
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STEFAN
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VICKI
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