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Revision as of 19:10, 10 October 2014
Wet Lab Journal
Week 1
Monday 23rd June
Make up 100ml of LB Broth and 100ml LB Agar.Make an overnight starter culture of BBa_K258008 to test sterile technique.
Tuesday 24th June
Generate Chemically competent E.Coli.Make up 8 flasks of 100ml starter culture.
4 flasks were checked each time to take the OD readings.
OD readings to show when the cells are in exponential growth phase and so ready to be made competent.
A | B | C | D | |
---|---|---|---|---|
1.25h | 0.077 | 0.078 | 0.082 | 0.096 |
3.25h | 0.567 | 0.674 | 0.714 | 0.809 |
Aliquot into 24 falcon tubes. The cells will need to be spun down in 2 rounds.
72 eppendorf tubes will be produced, labelled ch. comp, dh5alpha.
Store at -80°C.
Week 2
Monday 30th June
Make overnight starter cultures of the following;Tube | BioBrick | Antibiotic |
---|---|---|
1 | BBa_K258008 | Chloramphenicol |
2 | BBa_K215107 | Tetracycline |
3 | BBa_K861061 | Chloramphenicol |
4 | BBa_K215002 | Ampicillin |
5 | BBa_K1149021 | Chloramphenicol |
6 | BBa_K861060 | Chloramphenicol |
5μl of an appropriate antibiotic was added to each culture to allow selection for cells containing our biobrick plasmid.
Tuesday 1st July
Conduct 6 mini-preps, one for each of the biobrick cultures, to produce 6 Eppendorfs containing purified DNA.Wednesday 2nd July
Run a DNA gel using the purified DNA collected yesterday to check DNA is pure. Use option 3a.
Use an 8 well comb to produce the gel.
The table below shows the placement of each DNA sample within the Gel.
Well | Biobrick | Part Function |
---|---|---|
1 | 1kb gene ruler | |
2 | BBa_K1149021 | Promoter, RBS, Lipase |
3 | BBa_K258008 | ABC transporter |
4 | <BBa_K861060 | pFadR promoter |
5 | BBa_K861061 | pFadR Promoter + RFP |
6 | BBa_K215107 | ABC transporter (strong) |
7 | BBa_K215002 | pLAC +RBS +secretion signal + streptavidin binding tag |
The gel was run at 100v for 45 minutes (due to time constrains). Below is the image taken of the Gel on the Gel dock. 4 plates were made, 2 ampicillin and 2 chloramphenicol.
Nanodrop the DNA gained from the Mini-prep to generate concentrations of extracted DNA for all 6 biobricks.
Results are shown below;
Biobrick | Concentration |
---|---|
BBa_K1149021 | 115.0 |
BBa_K258008 | 075.9 |
BBa_K861060 | 100.3 |
BBa_K861061 | 130.7 |
BBa_K215107 | 043.3 |
BBa_K215002 | 125.0 |
Transform cells to ensuring competency
For this transformation We used the BioBricks BBa_K258008 and BBa_K215002 to check if the cells were competent.
Calculations are shown below;
BBa_K258008
75.9ng x X = 10ng x 100μl
X = 13.2μl
BBa_K215002
125.0ng x X = 10ng x 100μl
X = 8.0μl
Friday 4th July
The linearised Tlia and KerUS synthesised DNA is moved into a pJet1.2 plasmid using blunt end ligation.This ligation mix was then used totransform 3 eppendorfs of chemically competant cells (made on tuesday 25th);
Incubated for 45 minutes due to time constraints.
Constructs plated on ampicillin LB to select for the correct colonies.
Plates were checked on saturday AM and ...
Week 3
Monday 7th July
Make 200ml LB Agarand 200ml >LB Broth.Make overnight cultures of Tlia and KerUS.
Make overnight cultures of MC1000.
Tuesday 8th July
Miniprep the Tlia and KerUS cultures to produce purified plasmid DNA.Nanodrop the purified DNA to determine the concentration of DNA.
Concentration of DNA from plasmid mini-prep.
TliA - 5.2ng/μl
KerUS - 3.4ng/μl
Make chemically competent MC1000.
Measure the OD600 of the MC1000 cells using spectrophotometer
Flask 1 - 0.803
Flask 2 - 0.624
Blank - 0.066
Put 30ml MC1000 into falcon tubes. We have 4 tubes of full MC1000, the 5th one is 21ml MC1000 and 9ml water, the 6th one is all water.
Wednesday 9th July
Repeat yesterdays miniprep as it didn't yield enough DNA.Began with two 10ml starter cultures, one of Tlia and one of KerUS.
Decanted by hand into falcon tubes to give four 5ml cultures.