Team:Groningen/Project/Lab plan

From 2009.igem.org

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='''Lab plan:'''=
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{{Team:Groningen/Header}}
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=='''Lab plan:'''==
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For Basic Cloning strategy and final products see [https://2009.igem.org/Team:Groningen/Project The Project]
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# Clone gvp from BioBrick (BBa_I750016) in vector with inducible promoter (e.g. PAra)
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=='''Wk1 / Wk2'''==
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# Clone a metal ion transporter (CitM and HtmA are planned)
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For weekly of the lab work planning see [https://2009.igem.org/Team:Groningen/Notebook Notebook] --> Mondays
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# Clone a metal accumulating protein.
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# Clone a metal sensitive promoter in front of the gvp cluster.
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# Clone the metal accumulating protein and metal transporter in one vector, possibly on a synthetic operon
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# Transform both vectors in one ''E. coli'' strain
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=='''July:'''==
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=='''Gvp Cluster'''==
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For detailed planning of the labwork for different groups see the Construction phases in [https://2009.igem.org/Team:Groningen/Project_Plan Project Plan] for the functions Implementer and Tester (mostly combined for lab work)
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{{Team:Groningen/Footer}}
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*BBa_I750016 is a construct: E-genR-X-RBS-PART-S-P in vector BBa_J61035.
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*Possibly the AmpR and ColE1 are also still present on the vector, as the part was last checked in 2008 and contained a Amp resistance marker…
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*The part is present in the microtiter plate: Kit Plate 2, Well 11A
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*Quality control was okay, but plasmid length was different than expected. --> should be checked by us.
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*Plan:
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**Get chemically competent ''E. coli''
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**Dilute dry DNA of gvp with 15ul diH2O
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**Transform to ''E. coli'' --> see protocol
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**Plate on LB-A plates with Amp or Gentamicin selection (50/50)
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**Use positive and negative control
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**Grow o/n @ 37 degrees
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**Pick single colony and grow o/n in 5ml LB + correct antibiotic
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***Make glycerol stocks of the o/n culture
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***Do DNA isolation
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***Check the vectors insert by restriction analysis --> ''Pst''I and ''Xba''I (would give 1 band of ~ 3539bp and 1 of 6064bp)
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*Design primers to get rid of restrictionsites
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=='''CitM'''==
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*SJ transformed ''E. coli'' with pWSK29, a low copy nr vector containing CitM (according to B. Krom this is the best vector for CitM)
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*Get plasmid and possibly the plate with ''E. coli'' transformants.
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**Check expression of CitM while growing on citrate medium with Amp, induce with IPTG
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*Check gene for restriction sites and design primers to get rid of restrictionsites.
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*Design primers to introduce a pre/suffix --> ask B. Krom whether this would be feasible
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=='''HtmA'''==
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* On its way, but hopefully arrives next week
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=='''Accumulation of metal'''==
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*BioBrick (BBa_K129004) LamB + metal binding domain is not available
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*Find out whether it’s possible to only express the metal binding domain (6AA) and if so, order synthetic DNA with part with pre/suffix
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=='''To do list'''==
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*Get CitM from the biological centre
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*Finish equipment list --> send to facility manager
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*Design primers
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*Read articles to find [https://2009.igem.org/Team:Groningen/Project modeling parameters] for the different sub-projects and to find testing-phenotype (e.g. metal inport) protocols
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*Start ordering materials like: media, restriction enzymes, kits
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*Talk with Profs for permission to use stuff from the different groups in Haren
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Latest revision as of 11:03, 30 September 2009

[http://2009.igem.org/Team:Groningen http://2009.igem.org/wiki/images/f/f1/Igemhomelogo.png]

Lab plan:

For Basic Cloning strategy and final products see The Project

Wk1 / Wk2

For weekly of the lab work planning see Notebook --> Mondays

July:

For detailed planning of the labwork for different groups see the Construction phases in Project Plan for the functions Implementer and Tester (mostly combined for lab work)