From 2012.igem.org
July 2012
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August 2012
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September 2012
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October 2012
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Note from Dr. Haynes: Rohit, please transfer all of the Notebook entries from the OWW Wiki
http://openwetware.org/wiki/Haynes_Lab:Notebook/ASU_iGEM
To this page. Follow the format below. I added a couple of sections to help you get started.
June 07
Transformation (LSE)
Transformed DNA:
lacZ (well 4:12G, I732019)
p + lacO (well 1:6G, R0011)
Cells: neb10beta (donated)
Protocol from: http://www.neb.com/nebecomm/products/productc3019.asp
Controls: puc19, no DNA (8 plates)
June 08
Transformation results
puc19: growth
negative control: no growth
lacZ, lacO: possible small colonies
liquid culture in amp media (100 ug / ml):
no growth of lacZ, lacO
growth of puc19
June 12
DH5a Competent Cell Prep
Streak plated cells on LB no amp plate, let grow overnight
June 13
Transformation (LSE)
Transformed DNA:
lacZ (well 4:12G, I732019)
p + lacO (well 1:6G, R0011)
Cells: DH5 alpha (donated)
Protocol from: http://openwetware.org/wiki/Haynes:Assembly101 (30 minute transformation)
Controls: puc19, no DNA (8 plates)
Transformation (istb4, Abhi)
Transformed DNA:
Cells:
Protocol from:
Controls:
DH5a Chemically Competent cell prep
Grew 2 seed colonies from streak plate in LB no amp
Grew controls to test for contamination
Both Seed colonies grew, no contamination present
June 14
Competent cell prep
Prepared CaCl2 buffer solution and CaCl2 glycerol buffer solution
Grew seed colony in 400mL LB no amp
June 15
Competent cell prep
Centrifuged falcon test tubes containing liquid colonies
Resuspended in CaCl2 buffer solution and incubated for 15 mins
Centrifuged and resuspended in CaCl2 glycerol buffer solution
Chilled overnight
June 16
Competent cell prep
Aliquotted 200uL into test tubes
Stored in -80C
June 17
Streak plated prepared competent cells on LB no amp plate
June 19
Transformation (LSE)
Transformed DNA:
T7 promoter BBa_I712074
Constitutive promoter BBa_J23102
Cells: DH5 alpha (donated)
Protocol from: http://tools.invitrogen.com/content/sfs/manuals/subcloningefficiencydh5alpha_man.pdf (30 minute transformation)
Controls: puc19, no DNA
Plated 2 copies of each (100 ul, 250 ul) on LB amp plates.
Made 50 LB Amp plates.
June 20
Plated negative control on LB Amp plate
Liquid cultures of T7 promoter and constitutive promoter
Transformation (LSE)
Transformed DNA:
RBS (well 1:1H BBa_B0030)
TetR GFP (well 2:8A Part:BBa_I13522)
Cells: DH5 alpha (donated)
Protocol from: http://tools.invitrogen.com/content/sfs/manuals/subcloningefficiencydh5alpha_man.pdf (30 minute transformation)
Controls: puc19, no DNA
June 21
Made Liquid Cultures of E.coli transformed with RBS B0030
Made Liquid Cultures of E.coli transformed with TetR GFP
miniprepped and nanodropped T7 promoter BBa_I712074 and Constitutive promoter BBa_J23102 liquid cultures
liquid cultures:
RBS1
RBS2 (duplicate_
GFP1
puc19
negative controls
5 ml LB amp
overnight cultures
replated GFP1 & 2 (duplicates)
Nanodropped plasmid DNA samples
Constitutive promoter 1: __ng/uL
Constitutive promoter 2: __ng/uL
T7 promoter 1: __ng/uL
T7 promoter 2: __ng/uL
June 22
Miniprepped liquid cultures: RBS (well 1:1H BBa_B0030) and TetR GFP (well 2:8A Part:BBa_I13522)
June 26
Transformation:
Transformed DNA:
double terminator (B0017, 2:6K)
T7 RNA polymerase (I715038, 2:15C)
puc19, negative control
Protocol from: http://tools.invitrogen.com/content/sfs/manuals/subcloningefficiencydh5alpha_man.pdf (30 minute transformation)
Cells: dh5a
June 27
6-26 transformation results:
Controls correct
2x terminator: ~19 colonies
RNA pol: 1 colony
Liquid cultures including controls
June 28
Miniprepped double terminator (B0017, 2:6K) and T7 RNA polymerase (I715038, 2:15C) liquid cultures
July 2
Cleaned up liquid waste
Made SOB media
Finalized oligos for magainin construct
July 3
Autoclaved SOB media
Added glucose to make SOC media
Nanodropped double terminator (B0017, 2:6K) [DT1: 24.5, DT2: 29.6] and T7 RNA polymerase (I715038, 2:15C) [P1: 64.6, P2: 55.3] liquid cultures
July 24
Plasmids arrived courtesy of University of Pennsylvania School of Medicine
pET29a vectors containing coding sequence for Topoisomerase mutants CSCS and CSCS D168A described here
July 25
Tranformed CSCS topo 0 plasmid and CSCS D168A topo into DH5a Turbo cells (with neg control and Puc19 neg control)
Plated on Kanamycin plates