IGEM:UNAM Genomics Mexico/2009/Notebook/Wifi coli/2010/05/13: Difference between revisions
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===Goals for next week=== | ===Goals for next week=== | ||
*Search different copy number plasmid, with compatibility criteria. | *Search different copy number plasmid, with compatibility criteria. | ||
*Make a ligation between GFP-Reporter with plasmid. | *Make a ligation between GFP-Reporter with plasmid. | ||
*Make primers to get Lux AB genes from Vibrio Fischery. | *Make primers to get Lux AB genes from Vibrio Fischery. | ||
*Think about extraction of Lux CDE looking in registry parts how they made it. | *Think about extraction of Lux CDE looking in registry parts how they made it. | ||
*Make ligation for promoter and double terminator. | *Make ligation for promoter and double terminator. | ||
*Get Luciferase, get mutant and clone it | *Get Luciferase, get mutant and clone it. | ||
*Primers used for blue promoter: | *Primers used for blue promoter: BBa_K238013 | ||
==Modeling== | ==Modeling== | ||
Revision as of 17:14, 15 May 2010
 iGEM Project name 1
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13th may 2010WetLabExtraction of genomic DNA for blue promoter is done, but we don´t have amplified. Goals for next week
ModelingWe´ve got the primary function for activity of Luciferase and concentration of cytosolic Luciferin. =Goals for next week
Required data
propose, an association between promoter and quantity of reporter. Search protocols with measure about light and concentration. TRpR → aλ[P1] Promoter of Blue receptor → bλ[P2] Where λ is light. Ps, concentrations.
General
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