McGill/Team 1: Triple Ligation
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== July 2007 == | == July 2007 == | ||
=== July 5 === | === July 5 === |
Revision as of 01:11, 24 October 2007
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September 2007 | ||||||
Sa | Su | M | Tu | W | Th | F |
1 | 2 | 3 | 4 | 5 | 6 | 7 | 8 |
9 | 10 | 11 | 12 | 13 | 14 | 15 |
16 | 17 | 18 | 19 | 20 | 21 | 22 |
23 | 24 | 25 | 26 | 27 | 28 | 29 |
30 |
October 2007 | ||||||
Su | M | Tu | W | Th | F | Sa |
1 | 2 | 3 | 4 | 5 | 6 | |
7 | 8 | 9 | 10 | 11 | 12 | 13 |
14 | 15 | 16 | 17 | 18 | 19 | 20 |
21 | 22 | 23 | 24 | 25 | 26 | 27 |
28 | 29 | 30 | 31 | |||
Contents |
May 2007
May 14
- Made the same as May 15, but did not use Type 1 (milliQ) H2O, so the solutions were discarded.
May 15
- Made 1M CaCl2, and glycerol/CaCl2 solutions
- 1M CaCl2 Solution: 100mL was made
- CaCl2 Dihydrate = 146.986 g/mol
- 100mL of 1M CaCl2 requires 14.699g CaCl2 Dihydrate
- Glycerol/CaCl2 Solution: 30mL was made
- 5.00mL of 60% glycerol solution
- 3.00mL of 1M CaCl2
- 22.00mL of Type 1 (milliQ) H2O
- 1M CaCl2 Solution: 100mL was made
May 16
- Transformation of Cells:
- Transformed 1 vial of cells with Jun vector, and another vial with Fos vector (1uL of vector each); Sterile
- Used 400uL of LB (sterile) for each vial
- Incubated for 1 hour in shaker at 37C, then incubate overnight at 37C
May 30
- Test PCR Machine
June 2007
June 4
- Made Kanamycin plates
- 200mL of Agar
- 200mL of 2x LB
- 2mL of Kanamycin
June 20
Today: extract DNA from plates, transform, plate on amp plates.
I - Extraction of DNA from Plate (5M and 9G)
- Puncture foil with pippette tip
- Add 15uL of Type 1 water
- Remove all liquid (with DNA in solution)
II - Transformation of extracted DNA
- Chill cells on ice for 10 min
- Heat shock cells at 42°C for 30 sec
- Add DNA for cells
- Add 500uL of 42°C SOC medium to each vial
- Incubate on ice for 1 min
- Place in 37°C shaker incubator for 1h 30min
- Plate onto 4 separate amp plates
- 25uL R0062
- 25uL C0060
- 400uL R0062
- 300uL C0060
- Place into 37°C incubator at 3:55PM
Next: seed, miniprep and screen the DNA.
June 21
Checked colonies in the 37°C incubator. Well formed colonies were on each plate, so plates (all 4) were transferred to the small fridge (middle shelf on the right).
June 22
Today: miniprep DNA from July 20th transformation
I - Miniprep of Colonies from R25, R400, C25, C300 (indication the biobrick and the amount in uL that was plated)
- Transfer 1.5mL of cells suspended in LB into a microcentrifuge tube.
- Centrifuge for 2 min at max speed (14000 rpm)
- Remove supernatant with pipette and discard.
- Add 250uL of buffer P1 and 250uL of buffer P2
- Close and invert tubes 6 times
- Add 350 uL of buffer N3 (within 5 min of adding buffer P2)
- Close and invert 6 times
- Centrifuge for 10 min at 13000 rpm
- Carefully pipette off the supernatant into a Qiaprep spin column. NB: for sample R400 a large amount of supernatant was discarded. No reason, stupid move by Tim.
- Centrifuge spin column for 60 sec
- Discard flow-through
- Add 750uL of buffer PE
- Centifuge for 60 sec (max speed)
- Add 50uL of sterile water (of EB buffer could be used)
- Let stand for 1 min then centrifuge for 1 min
- Transfer flow-through to a new micro-centrifuge tube (one with a cap) with a pipette.
- Stored in -20°C freezer (green box labelled "Team 2")
- Remaining cells in LB stored in small fridge
Next: Screen the DNA.
June 26
Today: Screen of R0062 and C0060 from July 20th transformation
I - For R0062 add:
1.5uL of buffer 2
1.5uL of 10X BSA
3uL mini-prepped DNA
1uL of XmnI
1uL of XbaI
7uL of sterile water
Total volume = 15uL
II - For C0060
Same as above but no XbaI and 8uL water
Let both sit in 37°C water bath for 1h 40 min (From 3:30PM to 5:10PM)
III - Gel electrophoresis
- Add 12uL of water to each R25, R400, C25, C300
- Add 3uL of respective digested DNA
- Add 1.66uL of loading dye
- Gel contains:
- Ladder (5uL)
- R25 uncut
- R25 cut
- R400 uncut
- R400 cut
- C25 uncut
- C25 cut
- C300 uncut
- C300 cut
- The remaining uncut mini-prepped DNA was stored in the pink "Team 1" box.
Next: Interpret the screen and proceed to midi-prep or reseed.
June 28
Today: Reseeding of R0062
I - Reseeding of R0062
- Prepare 6 culture tubes with 2.5mL of sterile water and 2.5 mL of LB medium
- Add 5uL of 1000X Amp to 5 of the tubes (no antibiotic added to the control)
- 3 seedings from R25, 2 seedings from R400
- At 4:00PM the seedings were placed in the 37°C shaker incubator (in styrofoam pieces wedged inbetween clamps.
- Plates returned to fridge
Next: Miniprep and screen the re-seed.
June 29
Today: Digest and screen the re-seed from June 28th
I - Digest using same procedure as June 26th
- DNA was removed from the water bath at 4:35PM
II - Gel electrophoresis
- Gel contains
- Ladder (5uL)
- 400A
- 400B
- 25A
- 25B
- 25C
- Gel turned on at 5:02PM. 100V set for 40 min with variable current.
- Picture saved as "June 29 R400A R400B R25ABC"
Next: Interpret the gel and plan appropriate course of action.
July 2007
July 5
Today: Digest and screen R and C from July 4th midiprep
I - Digest Volumes
1.5uL 10X buffer
0.5uL suspended DNA (less than usual b/c midiprep is more conc.)
1uL EcoRI
12uL water
Total volume - 15uL
At 11:52AM tubes were placed in a 26.2°C water bath that was on its way up to 37°C.
II - Spectrophotometric DNA quantification
- Dilute DNA by a factor of 1000 (i.e. 1uL of DNA in 999uL of water). Mix by tapping.
- Reference (at 260 nm) a quartz cuvette that has been rinsed and filled with water.
- Rinse the cuvette with DNA solution.
- fill the cuvette and take an absorbance reading at 260 nm.
Results: A(R@260nm) = 0.022; a(C@260nm) = 0.75
Calculation: [DNA] = 50 x (dilution factor) x (Absorbance at 260nm)
Therefore [R] = 1100 ng/uL; [C] = 4250 ng/uL
Next: Gel quantification and ligation
July 25
Today: Sceening of Midi-prepped B0034
Only 0.5ul of Ladder was added because we were using syber-green. the load in other wells was: 1ul DNA, 1.67ul loading dye, 14ul water (total: 16.67ul)
The gel was loaded as:
- Ladder
- uncut B0034
- cut with XbaI
- cut with XmnI + BseRI
- cut with BseRI
- cut with XmnI
- cut with XmnI + XbaI
The gel was started at 3:36PM and run for 50 min. The gel picture was saved as "July 25 B0034 5 enz".
Next: Proceed with the next ligation.
July 27
Today: Turn off water incubator (37C) and placed in the freezer to stop the digest at 12:56PM. THe tube is in the pink Team 1 freezer box. (It's the only tube with tape on it.)
Next:Transform the ligation.
July 31
Today: Transformation of B0034+C0060 ligation.
August 2007
August 1
Today: Seeding of the B0034+C0060 ligation
I-Seeding
5 colonies from the 70ul plate and 5 from the 215ul plate (+2 controls)
Each tube contains:
- 2.5ml of 2X LB
- 2.5ml of distilled water
- 5ul Amp
Culture tubes placed in the 37C shaker incubator at 4:58PM. Plates were put back in the fridge (top shelf right hand side). NB: the 215ul had a cracked lid; the crack has been sealed with tape.
Next: Mini-prep and screen.
August 2
Today: Mini-prep of seeding from Aug 1
Digest carried out with EcoRI and SpeI in EcoRI buffer. The mini=prepped DNA was diluted by an extra 5ul of water during the digest so more DNA and less water was used when loading the gel (to ensure a decent resolution).
From the results of the gel we diluted 250ul of cells in suspension from tube 6f (215ul batch, #5) in 25 ml of LB and 25ul Amp, for Midi-prep.
The flask went into the SI (37C) at 6:15PM.
Next: Midi-prep.
August 3
Today: Midi-prep and screen
Note that the SI was turned off when Steph checked this morning, but there was growth, so we will proceed nonetheless. The Midi-prepped DNA was digested in two batches to ensure that everything worked properly.
Digest 1: BsrGI and SpeI with expected bands at 2455bp and 425bp.
Digest 2: BseRI and SpeI with expected bands at 2096bp and 784bp.
Digests were carried out in the 37C water bath starting at 12:23PM
We obtained unpromising results from the second digest. We suspect that the SpeI may be faulty, so we will try to cut it with BseRI and PstI. In buffer 2 PstI has only 75% efficiency so we will leave it overnight. Digest was started at 4:09PM.
After speaking with Jay we are going to try to regrow some cells left over from the original seeding (the 1 out of 10 that worked). There wa about 300ul left. We diluted 250ul in 25ml of LB. Cells went into the incubator at 5:26PM.
Next: Check on new digest and on cells in incubator.
August 4
Today: Check on new digest and on cells in incubator
Digesting DNA was taken out of the 37Cincubator at 11:08AM. BAD NEWS from the gel. Only one band b/w 3kb and 2kb and it wasn't a short band that ran off the gel, the smallest section of ladder was halfway down the gel. Picture is saved as "Aug 4 (BseRI + PstI)"
Removed
Also the bleach bottle is cracked and I didn't have time to switch it. Next: Check on new digest and on cells in incubator.
August 8
Today: Plating of B0034+C0060 (the second ligation attempt)
- Put Amp plates in the 37C incibator to warm them up at 2:25PM
- Plates went into the incubator at 3:23PM. Right Hand wall middle shelf
Next: Seed, mini-prep and screen
August 9
Today: Seeding and prepping reagents
I - [Preparation of 500ml of 2X LB]x2
II - Preparation of 200ml of agar
- 6g in 200 ml of water
III - 3 x 500ml of sterile water (type 2)
All went into the autoclave on setting 1 at 1:15PM
IV - Seeding of ligation: 250ul plate only
- Ten cultures (2.5ml LB, 2.5ml water, 5ul amp)
- Put into 37C shaker at 2:30PM
Note: the 25 ul plate had very abnormal growth so it was not seeded.
Next:mini-prep
August 10
Today: Mini-prep of 10 overnight cultures of ligated DNA
I - Cut with BseRI + SpeI and BseRI (if it needs to be redone, use PstI instead of SpeI). All 20 digests went into the 37C at 2:10PM
II - Gel electrophoresis
- We used 3ul of mini-prepped DNA, 12ul water, 1.66ul of loading dye
- In the way of results: 6 showed well in both, 3 showed well for the double digest but not the single cut, 8 showed well for the single but not the double
- All the same, we prepared midi-prep dilutions of all three (25ml LB, 250ul cells, 25ul amp) and we will screen the regrown cells before continuing.
- The dilutions went into the incubator at 6:40PM
Next:Midi-prep
August 11
Today: Midi-prep of dilutions of cultures 3, 6 and 8.
After midiprep the DNA was quantified spectrophotometrically.
3: 108 ng/ul
6: 30 ng/ul
8: 990 ng/ul
Due to the small amount of DNA from #6 we prepared another dilution in case it needs to be re-midi-prepped
I - Gel electrophoresis
- 8 cut with BsrGI one band at 3000bp
- 3 cut with BsrGI one band at 1300bp
- 8 cut with EcoRI + SpeI faint band at 3kbp others at 2kbp and 700bp
- 3 cut with EcoRI + SpeI one band 2kbp
File saved as "August 11 C+B midi screen digest"