Team:Czech Republic/Protocols
Protocols
Contents
Purification
Transformation (bacteria)
Transformation (yeast)
Gel electrophoresis
TBE stock 10X (1000ml)
- 108g Trisbase
- 55g Boric acid
- 9.3g EDTA (Ethylenediaminetetraacetic acid)
- dH20
- Add the ingredients into 900ml of dH20, mix it properly and fill to 1000ml.
- Store at room temperature.
NaOH stock 0,1M (200mL)
- 0.8g NaOH
- Boric acid
- dH20
- Add the ingredients into 200ml of dH20.
- Set pH on 8,5 by Boric acid.
- Store at room temperature.
Electrophoresis gel (100ml) 1%
- Agarose
- 1X TBE or 0,1M NaOH
- Ethidium bromide
Protocol:
- Add 0,7g agarose to 100ml 1X TBE or 10mM NaOH.
- Heat in microwave for 1 min at high power.
- Mix it and put it again into microwave for 1 min at high power.
- Make sure you have nitril gloves.
- Let it chill down for 6min and add 4 uL of ethidium bromide.
- Pour the balanced plate, don't forget to put the rake on.
- After the gel congeal, cover it with 1X TBE or 10mM NaOH.
For making small electrophoresis use half the amounts.
Miniprep
- Miniprep NucleoSpin Plasmid
- 2x 1.5ml eppendorf tube
Protocol:
- Overnight culture: Centrifuge 5ml at 11,000g for 30s, remove the liquid, add 250 uL A1 buffer, vortex properly and transfer it to the eppendorf tube.
- Petri dish: Add 250 L A1 buffer to the eppendorf tube, scrape off and add a culture from one partition, vortex properly.
- Add 250 uL A2 buffer (blue), gently invert 8 times, incubate for 5min at room temperature.
- Add 300 uL A3 buffer, gently invert to the change of colour (from blue to white).
- Centrifuge 7min at 11,000g.
- Transfer max 750 uL of the supernatant into 2ml spin column.
- Centrifuge 1min at 11,000g.
- Discard the flow-through and add 600 uL A4 buffer, centrifuge 1min at 11,000g.
- Discard flow-through and centrifuge 3min at 11,000g.
- Put the spin column into new eppendorf tube.
- Instil 25 uL DNA free water into the center of spin column filter, incubate for 3min at room temperature.
- Centrifuge for 1min at 11,000g.
- Repeat again steps 10-12.
Restriction digest
For a restriction digest of 500ng DNA, you need
- Restriction enzymes
- Corresponding NEB buffer
- 100X BSA
- XμL DNA (500ng)
- (42.5-X)μL dH2O
- 0.6mL tube
Protocol:
- Add appropriate amount od dH2O to the tube
- Vortex NEB buffer and add 5μL
- Vortex BSA and add 0.5μL (no need to add BSA when using NEB CutSmart buffer)
- Vortex DNA and add appropriate amount to the tube
- Vortex each enzyme and add 1μL to the tube
- Incubate at 37°C for 30min, then heat-inactivate at 80°C for 20min
- Store at 4°C
DNA Ligation
Insert mass in ng = \(3\frac{Insert\,length\,in\,bp}{Vector\,length\,in\,bp}Vector\,mass\,in\,ng\)
- 10X T4 ligase buffer
- 0.5uL T4 ligase
- Purified insert and vector (~50ng vector) DNA
- (8.5 - vector and insert)uL ultrapure dH20
- 0.6mL tube
Protocol:
- Add appropriate amount of ultrapure water to sterile 0.6mL tube.
- Vortex 10X T4 ligase buffer and add 1uL to the tube.
- Add appropriate amount of vortexed insert and vector DNA to the tube.
- Vortex T4 ligase and add 0.5uL to the tube.
- Place the tube in thermal cycler and run ligation protocol (60min incubation at 16°C, 10min at 65°C to denaturate the ligase)
- Store at -20°C
PCR Methods
Preparation of Primers
- Centrifuge a primer in the original tube.
- For 1 nmol of primer add 10 ul of DNA free H2O into original tube and vortex properly.
- Into new eppendorf tube add 24 ul of DNA free H2O, 3 ul of forward primer and 3 ul of reverse primer – work concentration
One Taq PCR protocol (25 ul reaction)
- Into PCR tube add 17,875ul of dH2O
- Add 5ul 5X One Taq Standard reaction buffer, 0,5ul dNTPs, 0,5ul of mix primers – work concentration, 1ul template DNA – work concentration 1 ng/ul and 0,125ul One Taq DNA polymerase.
Q5 PCR protocol
- Into PCR tube add 17 ul DNA free H2O.
- Add 5 ul 5X Q5 reaction buffer, 0,5 ul dNTPs, 1,25 ul of mix primers – work concentration, 1 ul template DNA – work concentration 1 ng/ul and 0,25 ul Q5 High-Fidelity DNA polymerase.
Adjustement of thermo cycler
- Denaturation – 10s, 98°C
- Annaeling - 30s, temperature depends on the primers
- Extension – time depends on the length of PCR construct - 30s for 1000bp, 68° for Taq / 72° for Q5
Band-stab PCR
Excellent technique when you want to amplify specific band from a gel. http://bitesizebio.com/13512/pcr-rescue/ More info..
- Prepare a complete 50μL PCR reaction without DNA template
- Take a sterile pipette tip and stab the desired band of interest 2-3 times
- Swirl the tip in the tube with prepared PCR reaction
- Run the PCR as usual
Gibson
Genome extraction
Soft lithography - PDMS molding
- Mix 40g of PDMS with 4g of curing agent
- Centrifuge the mixture at 3250 RPM for 3 minutes to remove the bubbles introduced during the mixing
- Clean silicon master with air gun
- Wrap an aluminium foil around the edges of the silicon master to create a container
- Pour the PDMS mixture over the silicon master
- Cure the PDMS in an oven at 80°C for 2 hours
- Leave the PDMS to cool down
- Detach the PDMS carefully from the silicon master
Soft lithography - Bonding PDMS-Glass
Preparation of the substrates
Glass slide
- Rinse the glass slide with acetone, isopropanol, and deionized water
- Dry the glass slide with air gun
- Dehydrate the glass slide on a hot plate at 120°C for 30 minutes
PDMS
- Slice the PDMS to individual PDMS replicas
- Drill holes for microfluidic inlets and outlets
- Clean the PDMS using a scotch tape
Air plasma treatment
- Place the glass slide and the PDMS replicas into a plasma cleaner, contact surfaces facing upwards
- Exhaust the atmosphere with a vacuum pump and wait until the pressure drops to 500 mTorr
- Activate the plasma for 2.5 minutes at Hi power
- Stop the plasma and open the valve to stabilize the pressure, continue immediately with the bonding phase
Permanent irreversible bonding
- Place the PDMS replica on the glass slide
- Place the bonded device in an oven at 80°C for 60 minutes.
- Seal the inlets and outlets with a scotch tape until use