Team:ESBS-Strasbourg/7 August 2008

From 2008.igem.org

Revision as of 09:54, 8 August 2008 by Paulo (Talk | contribs)
(diff) ← Older revision | Latest revision (diff) | Newer revision → (diff)

< back

Contents

DryLab

Modeling

WetLab

Paul
-recuperation of the overnight digest

-Gel migration and purification of the inserts c1/lacI/lexA/tetR/EYFP/adh1P/adh1t

-Dephosphorylation of the vectors containing respectively NLS/linker/Kozak sequences
precipitation phenol-chloroform and with alcool, resuspended in TE
vector +linker = 20µL (50ng/µL)
vector +NLS = 40µL (100ng/µL)
vector +Kozak = 500µL (50ng/µL)


-ligation for BB assembly:
ratio 1:3
1)c1/linker
2)lacI/linker
3)lexA/linker
4)tetR/linker
5)NLS/adh1-ter
6)EYFP/linker
7)adh1-prom/Kozak

ratio 1:8
respectively same construct than previously named
8/9/10/11/12/13/14

plates with only the vectors dP, no insert: linker/Kozak/NLS


-Transformation in LB plates + Amp, overnight

General

Quote of the day