Team:Paris Bettencourt/Notebook/Trojan Horse/Thursday 15th August.html
From 2013.igem.org
Trojan Horse
ASDF15th August
Place your twit here
Miniprep (Clovis)
pACY (pT002) : 109ng/uL
litmus (pT005) : 610 ng/Ul
Ligation (Aude, Clovis ,Vincent)
masse insert = ration (svt 10) * (taille insert / taille vecteur) * masse vecteur (50-100ng)
CHosen Vector mass = 50 ng
lacZ :
Digestion vector : 6,3 ng/ul
Digestion insert : 6,2
masse insert = 10*449/3770*50 = 59 ng
Protocol
Vector : 8 uL
Insert : 10 uL
Buffer : 2 uL
T4 DNA ligase : 0,2 uL
Let incubate at 22°C for 30 min
Kan :
Digestion vector : 7,8 ng/ul
Digestion insert : 12ng/ul
Insert mass = 10*1052/3770*50 = 140 ng
Protocole Ligation
Vector : 7 uL
Insert : 11 uL
Buffer : 2 uL
T4 DNA ligase : 0,2 uL
Transformation : (in chemical competent NEB turbo (made on the …) Aude Clovis
1) Thaw competent cells on ice.
These can be prepared using the CaCl2 protocol.
2) Add 5 ul of ligation product
4) Mix gently by flicking the tube.
5) Chill on ice for 30 minutes.
4) Heat shock at 42 °C for 30 seconds.
5) Return to ice for 2 minutes.
6) Add 300 ul LB medium and recover the cells by shaking at 37 °C for one hour
7) Plate on selective media
Plate on :
Tube 1 : negative control Xgal /IPTG /Cm ; Kan/Cm
Tube 2 : ligation lacZ-pacy (5uL) Xgal /IPTG /Cm
Tube 3 : ligation Kan-pACY (5uL) Kan Cm
Tube 4 : native plasmid (pACY) (1uL) Xgal /IPTG /Cm ; Kan/Cm
PCR (litmus = Backbone) Vincent
8 tubes, gradient 10°C around 64°C , started from a new miniprep
We see the plasmid => too concentrated
PCR (litmus pour la gibbson) Clovis
sTOO5 primer 005 006 protocol phusion (gradient around 64 + or – 5 °C)
Elongaiton time 2min10. Started with the new miniprep diluted.
Infectiveness characterization experiments (Vincent)
-the night before: prepare O/N of F+ cells, prepare O/N of phagemid producing cells (in this case : sT007 )
After checking GFP fluorescence of sT007 and its negative result, we decided to make a new sT007 glycerol stock. We used a colony from the first successful Infectiveness characterization experiments that was both AMP+KAN resistant and expressed GFP.
The following experiment was conducted with this new sT007 (strain MGZ1).
-centrifugate phagemid producing cells
-filter the supernatant 0.45um, stock it at 4°C (it contains the phages)
-This experiment was conducted both on MGZ1(F+) and MG1655(F+)
-dilute 200x MGZ1 and MG1655 from O/N
-wait until OD600 = 0.7
-immediately mix MGZ1 and the supernatant in different proportions
here we planned to try 1/10 (vol supernatant/vol cells)
-
1mL MGZ1,F+ + 100ul LB
-
1mL MGZ1,F+ + 100ul surnageant diluted 1/100
-incubate 45 minutes at 37°C for the protein to be expressed.
-
Serial dilute the tubes 10^-1, 10^-2, 10^-3, 10^-4, 10^-5, 10^-6
-
6 tubes with 900uL LB, add 100ul of one previously made tube, mix and transfert 100ul to next tube.
-
Plate on LB (10^-4 10^-5 10^-6), Kan(10^-1 10^-2 10^-3), Amp(10^-4 10^-5 - 10^-6), Kan and Amp(10^-1 10^-2 - 10^-3)