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Protocol
Miniprep
- Add culture medium 1mL in a microtube
- Centrifuge(1min,4°C,10,000rpm)
- Remove the supernatant to new microtube
- Repeat 1-3
- Add SolI 100μL and Vortex
- Add SolII 200μL and invert
- ice-cold 3min
- Add SolIII 150μL and invert
- ice-cold 3min
- Centrifuge(10min,4°C,10,000rpm)
- Add the supernatant to new microtube
- Add RNase 0.8μL
- Incubation(1h,37°C)
- Add phenol:chloroform 200μL
- Vortex
- Centrifuge(5min,4°C,10,000rpm)
- Add the supernatant to new microtube
- Add chloroform 200μL
- Tapping
- Centrifuge(1min,4°C,10,000rpm)
- Add the supernatant(150μL) to new microtube
- Add 3M-acetic acid 15μL
- Add 100%Et 400μL and invert
- Centrifuge(20min,4°C,10,000rpm)
- Remove the supernatant to new microtube
- Add 70%Et 400 μL
- Tapping
- Centrifuge(20min,4°C,10,000rpm)
- Remove the supernatant to new microtube
- Dry
- Add TE buffer 50μL
- Storage
Colony PCR
- Reagent
- TaKaRa Ex Taq(5units/μL) 0.5μL
- 10×Ex Taq buffer 10μL
- dNTP Mixture(2.5Meach) 8μL
- Primer F(10μM) 4μL
- Primer R(10μM) 4μL
- Template(E.coli DH5α)
- sterilized water(73.5μL)
- Conditions of the thermal cycler
- 95°C(2min)
- 95°C(30sec)
- 54°C(30sec)
- 72°C(40sec)
- 72°C(5min)
- 4°C(Save)
- 2-4:40cycle
- gradient:57-62°C(+0.1c)
Transformation
- Put competent cells on ice(10-15min)
- Add Ligation reaction solution(10μL) and tapping
- On the ice(30min)[Transformation]
- Add LB medium(0.7mL)
- Incubate(60min,37°C)
- Add X-gal(40μL) and ampicillin(10μL)[200μg/mL] on LB agar medium(IPTG)
- Add one incubated(100μL)
- Cultivation(overnight)
Ligation
- Reagent
- sterilize water 2μL
- PCR product 2μL
- vector DNA 1μL
- Ligation Mighty Mix 5μL
- Method
- Incubation(1h,16°C)
- Storage Overnight(-4°C)
Confirmed of electrophoresis by PCR product and Ligation of the TA vector
- Electrophoresis
- Gel concentration:1.2%,Migration time:30min
- Marker:Flash Gel 5μL
- Sample:dye 1μL,sample 5μL
- Check and Colony PCR
- Add to TA vector
- PCR product 2μL
- pMD20-Tvector 1μL
- D2W 2μL
- Ligation Mighty Mix 5μL
- Heat insulation(16°C,30min)
- Storage(-20°C)
The purified DNA
- Electrophoresis
- Marker:dye 1μL,DNA molecule 2μL,TE buffer 3μL
- Sample:dye 1μL,sample 5μL
- Gel concentration:1.2%,Migration time:30min
- Storage
PCR Product
- Electrophoresis
- DNA purification
- Confirmation of electrophoresis
- PCR
- Storage
Infusion
- Set up the In-Fusion cloning reaction:
- 5X In-Fusion HD Enzyme Premix 2 μl
- Linearized Vector x μl*
- Cloning Enhancer-Treated PCR Fragment x μl**
- dH2O (as needed) x μl
- Total Volume 10 μl
- *Use 50–200 ng of linearized vector.
- **Use 1–2 μl of Cloning Enhancer-Treated fragments, regardless of their length. The total volume of Cloning Enhancer-Treated PCR fragments should be up to 4 μl per 10 μl reaction. If you obtain a low product yield from your PCR reac¬tion, we recommend purification of PCR fragments instead of Cloning Enhancer-Treatment.
- Adjust the total reaction volume to 10 μl using deionized H2. 2O and mix the reaction.
- Incubate the reaction for 15 min at 50°C, then place on ice.
- Continue to the Transformation Procedure (Section VIII). If you cannot transform cells immediately, store the cloning reactions at –20°C until you are ready.
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