IGEM:UNAM Genomics Mexico/2009/Notebook/Wifi coli/2010/05/06

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=6th May 2010= =Advances=
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Modeling

 * Proportion/Bioparts (#Copies, promoter strength):  We need to take note about the efficiencies of

plasmids by systems. Problems with LRE, Lux Y and lumazine. LuxY and Lumazine, will be synthesized

with a strong promoter.


 * General formula (luminescence). Explain the general formula. Formula considers substrate-protein

concentration. The advantage of this formula is the literature related, in the article. Formula

includes cytosolic Luciferin. Formula lack of double luciferase activity.


 * Physical Design. Related 4 April, link image.


 * Team purposes make both physical designs, aisled (unidirectional) and open (multidirectional).


 * Limits. Quantity of L-cystein, for this we purpose a rich medium of L-Cystein.


 * Culture medium. Transparent, there are many options but in can be made.

We need:
Make a list for variables in model.

Re analyze the strength of promoter Vs copy number of plasmid.

Establish good proportions for concentrations in different bio-parts.

WetLab

 * WetLab partners are going on in constructions.

News

 * We will synthesize sequences in GenArt.

Plans

 * Exposition with instructors.


 * Ask for illuminometer.

Other stuff
Take note about importance of good Logbook.