Team:British Columbia/Notebook/Week 14

From 2011.igem.org

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===alpha-Pinene===
 
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Biobrick plasmids were sent to UBC NAPS sequencing. Results came back as a great sequence with Joe's illegal EcoRI site removed
 
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===alpha-Pinene===
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Biobrick plasmids were sent to UBC NAPS sequencing. Results came back as a great sequence with Joe's illegal EcoRI site removed
===Limonene Synthase===
===Limonene Synthase===

Revision as of 04:02, 29 September 2011

Team: British Columbia - 2011.igem.org

Week 14: Sep 4-10

Contents

Poster Making

Ubcigempostermaking.jpg
Ubcigemteamstrawberry.jpg
Joe, Daisy and Marianne got together one evening to work on the poster. We realized after we finished making the template for the poster that we have no data! Alina also came into give her input on the poster.

Later that night, Joe, Daisy, Marianne and Sam all went to Alina's lab to help her mash and pipet strawberry extract at 9 pm. A couple of Alina's lab members were also in the lab at 9 pm and were very surprised to find an illegal team of undergrads working on Alina's bench. PS We learned that Sam had a mullet and sang acapella at UCSF.



alpha-Pinene

Biobrick plasmids were sent to UBC NAPS sequencing. Results came back as a great sequence with Joe's illegal EcoRI site removed

Limonene Synthase

Ubcigemgcms2.tif

Joe and Alina went through some GC-MS data with Lina. We found out that the limonene synthase from the registry works! Read more about it on our data page.


Smiley Face C41 Competent Cells

Ubcigemsmiliecompetent.tif

Jacob has made more C41 competent cells for characterization of the synthases in bacteria.

Cineole Synthase

Disaster! Jacob returned from a couple of weeks vacation back in his home town in Manitoba to find that sequencing showed that his biobrick construction didn't work! A PSTI site remained in the original PGXE synthase, and when the restriction digest and ligation were done, it cut out the part after the site. The sequencing results from the other synthase gene (the PG) showed a tyrosine kinase, which, while interesting, was not what we wanted to send in. Jacob went back to using site directed mutagenesis to remove that site from his original plasmid, having learned that you want to be sure of the sequence of a part before putting it in biobricks.