Team:Uppsala/Experiments
Experiments and protocols
A majority of the protocols we used originate from the book "Synthetic biology-A lab manual", written by Anthony Forster, Erik Gullberg and Josefine Liljeruhm. They can therefore not be published here. We do however recommend you to buy it, as it was a great help in our project. The following protocols from the sixth chapter of this book were used:
- 0.9% NaCl
- 50% Glycerol
- 1M CaCl2
- 10x TBE Buffer
- SOB Medium
- LB Medium
- LB Agar Plates and Addition of Antibiotics
- Overnight Cultures with antibiotics, and glycerol stocks
- Agarose gel electrophoresis
- Preparation of competent E. coli cells using CaCl2
- Transformation of CaCl2 competent E. coli cells
- Bacterial re-streak techniques
- Digestion with DpnI
- 3A assembly
- Colony PCR
We also used several other protocols which we share below.
Biosurfactant characterization protocols
Drop collapse test
Materials required: 50mm petri plates, stop watch, olive oil and bacterial culture
Method:
- A 50mm petri plate was covered with 600 µl of olive oil.
- In the centre of the plate, small drops of either 50 or 100µl of bacterial culture were placed.
- The drop was observed for eventual collapse and the diameter of the drop was measured after 0, 5, 10, 15 and 20 min.
- A collapsed drop indicate that the presence of biosurfactants.
Thin Layer Chromatography
Materials required: Bacterial culture, 0.45 syringe filter, ethyl acetate, ethanol, chloroform, methanol, acetic acid, orcinol, sulphuric acid, hot air oven, vacuum centrifuge and TLC silica plates
Sample preparation:
- Overnight bacterial culture was centrifuged 10 000 rpm for 10 minutes.
- Supernatant of the samples were filtered using 0,45 μm syringe filter.
- The filtered supernatant was extracted with ethyl acetate in 1:1 v/v ratio three times.
- The organic solvent was removed by evaporation using vacuum centrifuge overnight.
- 10 μl 99% ethanol was added to the dried samples which then could be loaded on TLC silica plates
Sample preparation:
- TLC was performed using chloroform/methanol/acetic acid in a ratio of 65:15:2 as a developing solvent.
- For visualisation, the plate that has been developed was air dried and sprayed with a detection agent composed of 0.075 g orcinol, 4.1 mL sulphuric acid (60 %, v/v) and 21 mL deionised H2O.
- The plate was left to dry at room temperature, and then, the sugar moieties were stained by incubating the plates at 110 °C for 10 min.
CTAB plate recipe
Agar plate mineral salts medium: for 500 ml (pH 6.7)
- 10 g carbon source peptone per liter of distilled water
- 0.35 g KH2PO4
- 0.45 g Na2HPO4
- 1 g NaNO3
- 0.2 g MgSO4*7 H2O
- 0.05 g CaCl2*2 H20
- 1 ml of a trace elements solution (acidified with 37% HCl) containing 2 g FeSO4*7 H2O, 1.5 g MnSO4*H20, and 0.6 g (NH4)6Mo7O24*4H2O per-liter distilled water.
CTAB-methylene blue agar:
- 0.1g CTAB (cetyl-trimethyl-ammonium bromide)
- 0.0025 g methylene blue
- 7.5 g agar (difco) to 500 ml salts medium
Method: Preparation is similar to the preparation of LB agar plates