Team:NYU-AD/Notebook/Week3
Exterminator Coli
Week 3
26/07/2015
- The 3 transformation tubes containing Promoter2 + Ampicillin, Promoter3+Ampicillin, Promoter1+ Ampicillin, are still clean so we proceeded to discard them.
- After centrifuging the tubes, all the Terminator in Ampicillin tubes have white pellets except Ter2 tube (diluted), which had a red pellet. Hence we discarded Ter2 tube.
- We performed the Miniprep on the other 5 tubes with white pellets.
- Then performed digestion and ligation on the plasmids using standard protocols.
- Then we transformed the DNA into competent cells
Ligation
- Exception for the ligation:
- We added 5ul of each digest and ccdb backbone
- 2ul of DNA ligase
- 4ul of buffer solution but no water
- This was spun down for 10 seconds in the centrifuge.
Transformation:
- The transformation was done according to standard protocol
- However, for step 7, tube 1& 3 are placed in the normal incubator at 37˚C and at 130rpm
- However, for step 7, tube 1& 3 are placed in the normal incubator at 37˚C and at 130rpm
- We created 2 duplicates of transformation plate for each tube.
27/07/2015
- We did not use the correct restriction enzymes on the ccdb cells; hence we had to re-do the ligation and digestion of the plasmids. See above for the protocol ( for the 26/07/15)
- We then followed with the transformation of the plasmids by transforming 5ul each of the transformed plasmids in each tube of the competent cell
Transformation:
The transformation was followed according to standard protocol, with the exception of certain steps:
- Heat shock the cells at 42˚C.
- The cells were placed on ice for 3 instead of 5 minutes
- Pipette 900ul of S.O.C. mixture
- The tubes were shaken in the heating block at 37˚C, at 250rpm.
28/07/2015
For the stock concentration of antibiotic:
- we need 50ug/mL of Chloroamphenciol ( from earlier documentation)
- target conc: 50uh/mL
target conc: 50uh/mL - So we have 300ml of LB and our final conc. needs to be 50ug/mL. Hence we measure out 6mg of antibiotic into the broth.
- So We added 330ul of antibiotic ( of stock concentration 100mg/mL) into 300ml of LB Broth, then pipetted 10ml into each test tube.
- Picked colonies from each plate, inoculated them and left them in the incubator at 250rpm.
29/07/2015
- Miniprepped the plasmids but we accidentally threw out 2 test tubes of DNA but we still had 4 duplicates left.
- We then performed a Nanodrop of the ChiA constructs
Tube | Nucleic acid | Unit | A260 | A280 | 260/280 | 260/320 | Factor |
---|---|---|---|---|---|---|---|
ChiA 3.1 | 95.2 | ng/ul | 1.904 | 0.987 | 1.93 | 2.27 | 50 |
ChiA 2.1 | 37.0 | ng/ul | 0.741 | 0.379 | 1.96 | 1.82 | 50 |
ChiA 2.2 | 360.0 | ng/ul | 7.200 | 3.811 | 1.89 | 2.26 | 50 |
ChiA 3.2 | 156.3 | ng/ul | 3.127 | 1.646 | 2.02 | 1.91 | 50 |
26/08/2015
- Performed ligation of the promoter and tnaA
- Amplifying the tnaA and tnaB sequence.
- Added 200ul of water (DNA- RNA free) into each tube
- Performed the Nano Drop . The concentration of both tubes is approximately 7-8ug/ul.
27/08/2015
- Nanodrop to verify concentration of resuspended DNA
- Nuclease- free H2O used to resuspend the DNA was found to be contaminated with 4.8ug/ul of DNA
- The actual DNA content of plasmids are around 6-8 ug/ul on average
- We decided to proceed with the transformation since protocol specified 10ug- 100ug of DNA.
30/08/2015
- We made liquid broth, Kanamycin
Preparing agar plates:
- Take 35g of agar powder in 1L of solution.
- Add the powder then autoclave the solution( 1hour)
- We already have antibiotic stock solution of 100mg/ml
Note: Due to coagulation, we had to put in 400ul of antibiotic( chloroamphenicol) instead of 500ul as originally desired.