Team:Czech Republic/Protocols

Protocols

Contents

1 Purification
2 Transformation (bacteria)
3 Transformation (yeast)
4 Gel electrophoresis
5 Miniprep
6 Restriction digest
7 Band-stab PCR
8 Gibson
9 Genome extraction
10 Soft lithography - PDMS molding
11 Soft lithography - Bonding PDMS-Glass
12 ...

Purification

Transformation (bacteria)

Transformation (yeast)

Gel electrophoresis

Miniprep

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

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

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