Team:UCL/Labbook
From 2013.igem.org
June
Week 1-3
No lab work
Week 4
26th June - We are given safety training in the Advanced Centre for Biochemical Engineering in all relevant laboratories, as well as general procedures in case of emergency.
July
Week 5-6
No lab work
Week 7
Bacterial Lab
15th July - The team is introduced to the laboratories which will be used during the summer for both bacterial and mammalian experiments. 16th July - 5X M9 salts [link to protocol], minimal agar [link to protocol], 1.4% molten agar solution [link to protocol] and 0.1M CaCl2/15% glycerol [link to protocol] were prepared for the generation of competent cells. Minimal agar plates were poured and streaked [link to streaking protocol] with W3110 Escherichia coli cells and left overnight to incubate at 37C. 17th July - Very little colony growth was observed from W3110 E.coli streaked plates. Plates were therefore left to incubate for a further 17 hours. 18th July - Sufficient colony growth allowed for the selection of a single colony from each plate. This was then inoculated in 5ul LB media [link to LB recipe] + 100ul 1M MgSO4 and left to incu-shake overnight at 37C. 19th July - Cultures re-suspended in new LB media and 100µl aliquots placed into individual eppendorf tubes for placement at -80C. Mammalian Lab 17th July - Mammalian cell culture and maintenance [link to mammalian protocol] training by Mrs. Ludmilla Ruban. Passaged primary MEF (mouse embryonic fibroblast) cells. Passage 3. 18th July - MEF passage 4 19th July - MEF passage 5Week 8
Bacterial Lab
22nd July -Transformation [link to transformation protocol] of our competent cells with plasmid YB3110 was carried out. 23rd July - No colony growth was observed on Ampicillin plates [link to ampicillin plate protocol] indicating no plasmid uptake. Transformation was repeated with YB3110.Vial | Ampicillin Plate | Plasmid Insertion | Colony Count |
---|---|---|---|
1 (Main) | Yes | Yes | 0 |
2 (Positive Control) | No | Yes | 100+ |
3 (Negative Control) | Yes | No | 0 |
Vial | Ampicillin Plate | Plasmid Insertion | Colony Count |
---|---|---|---|
1 (Main) | Yes | Yes | 0 |
2 (Positive Control) | No | Yes | 100+ |
3 (Negative Control) | Yes | No | 0 |
Vial | Ampicillin Plate | Plasmid Insertion | Colony Count |
---|---|---|---|
1 (Main) | Yes | Yes | 0 |
2 (Positive Control) | No | Yes | 100+ |
3 (Negative Control) | Yes | No | 0 |
Vial | Ampicillin Plate | Plasmid Insertion | Colony Count |
---|---|---|---|
1 (Main) | Yes | Yes | 0 |
2 (Positive Control) | No | Yes | 100+ |
3 (Negative Control) | Yes | No | 0 |
Week 9
Bacterial Lab
29th July - A glycerol stock of pSecTag2A from 2009 was restored. This was streaked onto 3 plates (2x LB Amp and 1x No drug), additionally four Falcons with 2ul LB were inoculated with the glycerol stock (2x LB No drug, 2X LB Amp). These were left to incubate overnight. 30th July - pSecTag2A Amp and No drug cultures were centrifuged (5 minutes at 4000rpm) and the pellet frozen to be used later in a miniprep. pSecTag2A plates displayed good colony growth. Colonies were picked from non-competent W3110 streaked plates and inoculated in LB ->incu-shake 37C o/n.Vial | Ampicillin Plate | Plasmid Insertion | Colony Count |
---|---|---|---|
1 (Main) | Yes | Yes | 100+ |
2 (Positive Control) | No | Yes | 100+ |
3 (Negative Control) | Yes | No | 0 |
Item | Volume (ul) |
---|---|
DNA pSecTag2A | 5 |
HindIII | 1 |
Buffer | 1 |
BSA | 0.5 |
dH20 | 2.5 |
Total | 10 |
August
1st August - Results from newly generated competent cells transformed with pSecTag2A:Vial | Ampicillin Plate | Plasmid Insertion | Colony Count |
---|---|---|---|
1 (Main) | Yes | Yes | 100+ |
2 (Positive Control) | No | Yes | 100+ |
3 (Negative Control) | Yes | No | 10 |
Vial | Ampicillin Plate | Plasmid Insertion | Colony Count |
---|---|---|---|
1 (Main) | Yes | Yes | 100+ |
2 (Positive Control) | No | Yes | 100+ |
3 (Negative Control) | Yes | No | 15 |
Week 10
Bacterial Lab
5th August - The new batch of ampicillin was tested via transformation of competent cells with pSecTag2A. Plates were spread and incubated 37C o/n. 6th August - Results from yesterday’s transformation:Vial | Ampicillin Plate | Plasmid Insertion | Colony Count |
---|---|---|---|
1 (Main) | Yes | Yes | 100+ |
2 (Positive Control) | No | Yes | 100+ |
3 (Negative Control) | Yes | No | 15 |
Vial | Ampicillin Plate | Plasmid Insertion | Colony Count |
---|---|---|---|
1 Old Ampicillin | Yes | Yes | 100+ |
2 New Ampicillin v2 | No | Yes | 100+ |
3 Positive Control | Yes | No | 15 |
Week 11
Bacterial Lab
12th August - Chloramphenicol [link to Chloramphenicol recipe] was produced and stored at -20C. In order to produce glycerol stocks, pSecTag2A and pSB1C3 were inoculated with LB media in two falcon tubes each (1x drug, 1x no drug), two plates for each plasmid were also streaked (1x drug, 1x no drug). All were left to incubate at 37C o/n. 13th August - Results from the following plates:Vial | Ampicillin Plate | Plasmid Insertion | Colony Count |
---|---|---|---|
pSecTag2A Cells | Yes | Yes | 100+ |
W3110 Cells Amp | Yes | No | 0 |
pSecTag +ve control | No | Yes | 100+ |
PSB1C3 Cells | Yes | Yes | 0 |
W3110 Cells Chlor | Yes | No | 25 |
PSB1C3 +ve control | No | Yes | 0 |
Item A | Volume A (ul) | Item B | Volume B (ul) |
---|---|---|---|
pSecTag2A | 5 | pSecTag2A | 5 |
EcoR1-HF | 1 | Dpn1 | 1 |
Buffer 4 | 1 | Buffer 4 | 1 |
BSA | 0.5 | BSA | 0.5 |
dH20 | 2.5 | dH20 | 2.5 |
Total | 10 | Total | 10 |