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Team:SCAU-China/Methods & Materials
From 2014.igem.org
Methods and Materials
MEDIUM
•LB medium- Tryptone 10 g/L
- Yeast Extract 5 g/L
- NaCl 10 g/L
•SOC medium
- Tryptone 20 g/L
- Yeast Extract 5 g/L
- NaCl 0.50 g/L
- KCl 0.18 g/L
- MgCl 0.59 g/L
- Glucose 3.6 g/L
MFC performance assay
1.Prepare anode medium, cathode medium and MFC device, autoclave at 115℃ for 15 min.2.Inoculate E.coli at 37℃ overnight until optical density (OD600nm) reach 2.0
3.Centrifuge at 25℃, 5000 rcf, 5 min discard supernatant and resuspend bacteria with 100 mL anode medium solution.
4.Fill the anode chamber with anode solution and seal with rubber plug. Pour 60~80 mL cathode medium into cathode chamber until the proton exchanging membrane (PEM) being overwhelm.
5.Load a 1,000 Ω resistor into the circuit, and connect to the digital multimeter with recorder.
6.Incubate the chamber overnight at 37℃.
Medium for MFC
•Anode medium| Ingredient | Concentration |
|---|---|
| glucose | 2.0 g/L |
| NH4Cl | 0.25 g/L |
| KCl | 0.1 g/L |
| trace element solution | 10 mL |
| PBS buffer (Na2HPO4 and NaH2PO4) | 50 mM |
| riboflavin | 100 μM |
| Ingredient | Concentration (g/L) |
|---|---|
| MgSO4•7H2O | 3.0 |
| MnSO4•H2O | 0.5 |
| NaCl | 1.0 |
| FeSO4•7H2O | 0.1 |
| CoCl2•6H2O | 0.1 |
| CaCl2 | 0.1 |
| ZnSO4•7H2O | 0.1 |
| CuSO4•5H2O | 0.01 |
| KAl(SO4)2•12H2O | 0.01 |
| H3BO3 | 0.01 |
| Na2MoO4•2H2O | 0.01 |
50mM PBS
Constructs through Ω-PCR
1.design primers containing overlap sequences.2.1st Ω-PCR
3.Exo I digest at 37 ℃ for 20 min.
4.2nd Ω-PCR
5.Dpn I digest at 37 ℃ for 1 hour.
6.Dialysis for 30min
7.Transform into electrocomponent cells
•1st Ω-PCR mixture
| For 1 reaction | Final concentration | |
|---|---|---|
| 2x PCR buffer for KOD FX | 10 μl | 1 × |
| 2mM dNTPs | 4 μl | 0.4 mM each |
| 10μM Primer #1 | 0.4 | 0.2 μM |
| 10μM Primer #2 | 0.4 | 0.2 μM |
| Genomic DNA ~200 ng / 50μl | ||
| Template DNA | ≧ 1 μl | Plasmid DNA ~50 ng / 50μl cDNA (from ~200 ng RNA) / 50μl |
| KOD FX (1.0U/μl) | 0.4 μl | 1.0 U / 50 μl |
| Autoclaved, distilled water | up to 20 μl |
PCR cycle condition
| Step | Temp | Time |
|---|---|---|
| 1:Predenature | 94 °C | 4 min |
| 2:Denature | 98 °C | 15 s |
| 3:Annealing | (Tm-5)°C | 30 s |
| 4:Extension | 68 °C | 1min/kb DNA |
| 5:Go To step 2 | / | 35 cycles |
| 6:Final Extension | 68 °C | 10 min |
| 7:Storage | 4 °C | ∞ |
•2nd Ω-PCR mixture
| For 1 reaction | Final concentration | |
|---|---|---|
| 2 x PCR buffer for KOD FX | 10 μl | 1× |
| 2mM dNTPs | 4 μl | 0.4 mM each |
| 1st Ω-PCR product | ≥1 μl | 50~400 ng |
| Template plasmid | ≥ 1 μl | 5~100 ng |
| KOD FX (1.0 U/μl) | 0.4 μl | 1.0 U / 50 μl |
| Autoclaved, distilled water | up to 20 μl |
PCR cycle conditions
Arca knockout method
1. Transfer plasmid pKD46 into the wild type E. coli MG1655; screen the positive colony using Ampicillin.2. Use pKD46 specific primers to screen transformants by colony PCR.
3. Prepare pKD46 positive electrocomponent cell.
4. Amplify Kanamycin resistant gene NPTII using primer 1 and 2.
5. Purify the NPTII fragment by electrophoresis.
6. Transfer the NPTII segment into the wild type cell with pKD46.
7. Screen Kan and Amp resistant strain on selection media.
8. Use PCR (primer 3 and 4) to confirm the arcA knock-out colony.
9. Sequencing the target gene to confirm the knock-out effect.
Primer 1 gacttttgtacttcctgtttcgatttagttggcaatttaggtagcaaacatgagccatattcaacggga
Primer 2 ataaaaacggcgctaaaaagcgccgttttttttgacggtggtaaagccgattagaaaaactcatcgagca
Primer 3 gtcatgttacgccgatcatg
Primer 4 ttgggaaccagtgtgctggt
Confirming PCR reaction mixture
| Component | Volume (μl) |
| ddH2O | 13 |
| 10 x PCR buffer | 2 |
| dNTP mix | 0.4 |
| Primer 3 | 0.4 |
| Primer 4 | 0.4 |
| Taq polymerase | 0.4 |
| Bacteria | 3 |
Amplification PCR reaction mixture
| Component | Volume (μl) |
| ddH2O | 160 |
| 10 x PCR buffer | 20 |
| dNTP mix | 4 |
| Primer 3 | 4 |
| Primer 4 | 4 |
| Taq polymerase | 4 |
| DNA template | 4 |
