Team:Calgary/11 June 2009
From 2009.igem.org
CAROL
Descriptive Title of What You’re Doing
WIKI CODING HERE
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CHINMOYEE
CLASS
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EMILY
Gradient PCR Take Two
File:2009.06.12.LuxOD47E Gradient PCR.tif
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FAHD
Marketing for June 11th 2009
Today, we gad a meeting with Derek Gratz who is a University of Calgary Alumni and the owner of WestLink Innovations. He gave us good ideas on how to approach companies and how to important it is to build a network with these companies. He also gave us names of a few potential companies that might be interested in our project
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IMAN
Descriptive Title of What You're Doing
WIKI CODING HERE
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JAMIE
Descriptive Title of What You're Doing
WIKI CODING HERE
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JEREMY
Descriptive Title of What You're Doing
WIKI CODING HERE
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KATIE
Success
I was able to combine all three scripts into one by using the listen event and now it is possible for me to add more types of DNA to PCR and I can continue to easily add quite a few of them. I also was able to fix the error I was getting, which happened because as long as the first item stored in a list was found in the machine’s inventory, it believed everything was there, but when it went to do something with it, the item did not exist and an error occurred.
However, I would still like to change the way it is being used at this time since it is not really efficient to re-declare a variable every time you go through a loop. I will work on changing this at a later date.
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KEVIN
Plasmid Isolation of LuxCDABE (luciferase)
The LuxCDABE is being isolated by Caron Chan, but she needed some hands on this, and I was willing to help. LuxCDABE was isolated with Quigen's EndoFree Plasmid Maxi (quigen) according to the specification of the provider. A different kit than the one used in previous experiments was used because the LuxCDABE is very big in size (6kb), and the Minprep would not be capable of isolating the plasmid at a high enough concentration.
Despite of the use of Maxiprep, however, the spectrophotometer seemed to have not picked up any plasmid in the isolated sample, as the purity and concentration were below acceptable. Another Maxiprep may be needed to be done. |
MANDY
Descriptive Title of What You're Doing
WIKI CODING HERE
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PATRICK
Physical Objects and Nonphysical Objects Do Not Get Along
Retrospective Notebook: This entry was not written on this day, but derived later from working notes I made that day.
Began setting up a workaround for the problems with using SL's 'collision' event for object messaging. First started changing the object movement script to toggle its 'physics' state on and off, instead of continuously setting its velocity to zero, which would be a much smoother and simpler solution to that problem. I had by this time built a working RNAP, insofar as it would bind at the promoter, follow the DNA and detach at a terminator. I also encountered a problem with the RNAP polymerase and the DNA in collision, where because the DNA object was physical (ie, subject to the physics engine in second life) but the RNAP was not physical (so that it could occupy the same space as the DNA without colliding with it), the RNAP would try to move along the strand of DNA, but wound up 'pushing' the movable DNA along. If left alone, this setup would continue crawling across the world indefinitely! Ultimately, when two objects have to live in close proximity with each other, they must both be set to nonphysical or they will exhibit collision glitches like this.
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PRIMA
WestLink Innovations Meeting
Fahd, Thane and I went to meet the President from WestLink Innovations.He offered advise on how to contact companies, what to say, what not to say, who we should contact. He offered to help us with networking. It was nice of him to take time out of work to meet and discuss marketing strategies with us.
What I got out of this:
1) Contact information for other companies
2) names to new companies which I hadn't thought of
3) established a relationship between iGEM and WestLink Innovations
4) Advice on marketing emails + follow up phone calls
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STEFAN
Descriptive Title of What You're Doing
WIKI CODING HERE
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VICKI
Re-do of gradient PCR because of contamination issues
Purpose: The last gradient PCR for BioBrick amplification failed because of contamination. This is the second attempt.
Materials and methods: Please refer to the June 4th entry for the observed protocol. Results: Shown below, with the lane key included. The blank negative control lane is reassuring. The ladder is a GeneElute 1kb Plus DNA ladder.
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