Team:Cambridge/LabBook/Week9
From 2010.igem.org
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+ | PCR | ||
+ | |||
+ | *Denaturation: 5min @ 98°C | ||
+ | *35 cycles: | ||
+ | **12s @ 98°C : Denaturation | ||
+ | **20s @ 58°C : Annealing | ||
+ | **20s @ 72°C : Elongation | ||
+ | *Elongation: 5min @ 72°C | ||
+ | *Hold at 10 | ||
+ | |||
+ | Touchdown PCR | ||
+ | |||
+ | *10 cycles | ||
+ | **Denaturation: 12s @ 98°C | ||
+ | **Annealing: 20s @ 65 to 55°C | ||
+ | **Elongation: 20s @ 72°C | ||
+ | |||
+ | *35cycles | ||
+ | **Denaturation: 12s @ 98°C | ||
+ | **Annealing: 20s @ 55°C | ||
+ | **Elongation: 20s @ 72°C | ||
+ | |||
+ | *Elongation 5min @ 72°C | ||
+ | |||
+ | We then ran a gel | ||
+ | |||
+ | Products were obtained for strain 2 in both Touchdown lanes and in one normal PCR lane | ||
+ | |||
+ | |||
µl°C | µl°C |
Revision as of 11:10, 29 September 2010
Contents |
Monday
86. Expt: Extract CDABEG from pJS555
- Using 2 primers
- prefix start of O
- suffix end of G
- Hope that it will glow in its own right without luxR+I
- Need to put under a new promoter
87. Expt: Gibson transformation (cont. from p.70)
3 colonies on one plate were not pink. These were streaked out on new Chl plated and put into liquid cultures along with 2 of the red colonies.
Next check for the right sized fragment with colony PCR and try to induce with arabinose.
88. Expt: Plate Reader G28
Well | Arabinose conc. | |
A1 | 0 | x1,9 |
A2 | 1µM | |
A3 | 5µM | |
A4 | 10µM | |
A5 | 100µM | |
A6 | Blank | |
A7 | pSB1C3 | |
A8 | Blank | x8,16 |
Reads every 10 mins
89. Expt: Extracting YFP, CFP, Luc tetR, G28 via miniprep (Paul)
Nanodrop readings (ng/µl) | ||
YFP | 33.3, 55.4 | |
CFP | 17.9, 20.4 | |
Luc tetR | 33.7 | |
G28 | 125.3, 96.9 | |
G28? | 17.9 |
90. Expt: Colony PCR to extract the thioesterase gene from E. coli K12 (Paul)
We used TOP10 cells, a substrain of DH10B, which is a substrain of K12.
We did a colony PCR to isolate the gene:
3 replicates with: | 1 negative control: | |
2x Phusion Mastermix | 10µl | 10µl |
Template DNA | 1µl | 0 |
Primer 1 | 1µl | 1µl |
Primer 2 | 1µl | 1µl |
Nuclease-free H20 | 7µl | 8µl |
The negative control was to check for primer/dimer and contamination.
PCR protocol:
- Initial denaturation: 5min @ 98°C
- Touchdown: 16 cycles
- Denaturation: 10s @ 98°C
- Annealing: 20s @ 65°C to 57°C
- Elongation: 15s @ 72°C
- 30 cycles
- Denaturation: 10s @ 98°C
- Annealing: 20s @ 50°C
- Elongation: 15s @ 72°C
- End and hold at 10°C
- We then ran result on a gel with SyberSafe at 6x lodaing Dye and Hyperladder IV
Lane: 1 | 2 | 3 | 4 | 5 |
Ladder | Tube 1 | Tube 2 | Tube 3 | Negative Control |
Failed: Something obtained in control...
Nothing in other lanes
We repeated without touchdown PCR:
- Denaturation 5min @ 98°C
- 35 Cycles
- Denaturation: 12s @ 98°C
- Annealing: 20s @ 58.5°C
- Elongation: 15s @ 72°C
- Hold at 10°C
Failed again: Product in negative control observed again...
Tuesday
91. Expt: Further testing
Column | Arabiniose/µl | Well names | ||
Repeat 1 | Repeat 2 | Repeat 3 | ||
1 | 0 | X1 | X12 | X23 |
2 | 0 | X2 | X13 | X24 |
3 | 0 | X3 | X14 | X25 |
4 | 5 | X4 | X15 | X26 |
5 | 10 | X5 | X16 | X27 |
6 | 50 | X6 | X17 | X28 |
7 | 100 | X7 | X18 | X29 |
8 | 1000 | X8 | X19 | X30 |
9 | 10,000 | X9 | X20 | X31 |
10 | Blank | X10 | X21 | X32 |
11 | Blank | X11 | X22 | X33 |
Inoculation: 1ml overnight added to 3ml, Amp + Cm
92. Expt: Restriction Enzyme Digests
DNA | Enzymes used | Subsequent Nanodrop readings/ng/µl | |
1. | Linear Plasmid | EP | 5.6 |
2. | Luc TetR | ES | 4.0 |
3. | Luc TetR | EP | 2.8 |
4. | RBS YFP | XP | 19.4 |
5. | RBS CFP | XP | 2.9 |
6. | G28 lux | SP | 6.1 |
93. Expt: Extracting DNA 2.0 from Registry
- Remove filter from plastic bag and place on a sterile and clean surface.
- Add 100µl of 10mM Tris-HCl, pH 7.5 directly to the center of the filter
- Incubate at room temperature for 2minutes.
- Puncture the bottom of at 0.6ml tube using a syringe.
- Place filter in the 0.6ml tube and place 0.6ml tube in a 1.5ml tube.
- Place the 1.5ml tube(now containing punctured 0.6ml tube with filter) in tabletop centrifuge.
- Spin 1 minute at full speed. The DNA containing liquid will transfer from the filter in the 0.6ml tube into the 1.5ml tube.
- Discard the 0.6ml tube with filter. The 1.5ml tube now contains ~90µl buffer+DNA.
- Carefully remove supernatant. there may be a small pellet consisting of filter debris. This pellet does NOT contain any of the DNA. The supernatant should contain approximately 2µl plasmid DNA(~20ng/µl).
The isolated DNA can subsequently be transformed, cut with restriction enzymes, or sequenced without further purification.
Then transformed using standard protocol
Result: Colonies all grew
Wednesday
94. Expt: Ligating restriction digests from yesterday
Theo wished to prepare three constructs:
- A: P[TetR repressed] - WT luciferase - YFP in pSB1C3
- B: pBad Lux aoperon (G28) - YFP in pSB1C3
- C: P[TetR repressed] - WT luciferase
Volumes all in µl
pSB1C3 linearised cut with EP. | Luc cut with ES. | Luc cut with EP. | G28. | YFP. | Rapid ligation buffer. | T4 ligase. | |
A | 4 | 9 | 0 | 0 | 2 | 4 | 1 |
B | 4 | 0 | 0 | 9 | 2 | 4 | 1 |
C | 2 | 0 | 13 | 0 | 0 | 4 | 1 |
Theo then incubated for 5mins at 22°C and following transformation protocol, plating out on Chlor plates.
95. Expt: Colony PCR of cells transformed with the Gibson assembly product (pages 70,73) (Done by Peter)
Took 2 colonies of plates ABCDE each
ran PCR on G-storm ('Phusion Lng rng clny PCR')
27 cycles
- melting: 98µl 15s
- annealing: 60µl 10s
- extension: 72µl 3min
final elongation 10min
Ran on E-gel:
faint band at ~2000bp
no band visible at the expected 6.6kbp
PCR tubes placed in Freezer, ~30µl left
96. Expt: Colony PCR to extract the thioesterase gene from E. coli K-12 (repeat using new protocol)
We used K-12 strains from Veio collection ( JW3582 and JW5313) but during the cell lysis protcols writing on tubes was erased so we couldn't identify the 2 strains.
Cell lysis
- Heat at 98 for 10 min
- Freeze at -80 for 10min
- Vortex for 2min
Cells were collected from plates and put in 20 of dH20
We performed 2 PCR (normal and touchdown) with 2 replicates for each strain and one negative control:
negative control | |
7µl of dH20 | 8µl of dH20 |
10µl of 2x Phusion Mastermix | 10µl of 2x Phusion Mastermix |
1µl of primer 1 @0.5mM | 1µl of primer 1 @0.5mM |
1µl of primer 2 @0.5mM | 1µl of primer 2 @0.5mM |
1µl of Cell suspension |
PCR
- Denaturation: 5min @ 98°C
- 35 cycles:
- 12s @ 98°C : Denaturation
- 20s @ 58°C : Annealing
- 20s @ 72°C : Elongation
- Elongation: 5min @ 72°C
- Hold at 10
Touchdown PCR
- 10 cycles
- Denaturation: 12s @ 98°C
- Annealing: 20s @ 65 to 55°C
- Elongation: 20s @ 72°C
- 35cycles
- Denaturation: 12s @ 98°C
- Annealing: 20s @ 55°C
- Elongation: 20s @ 72°C
- Elongation 5min @ 72°C
We then ran a gel
Products were obtained for strain 2 in both Touchdown lanes and in one normal PCR lane
µl°C