Team:Tokyo Metropolitan/Notebook

From 2011.igem.org

Tokyo Metropolitan Labnotes.png

Contents

1 Lab Notebook
2 Lab Protocols

Lab Notebook

Lab Protocols

PCR (PrimeSTAR® HS DNA Polymerase)

Ice
Micro pipette
Thermal cycler
PCR Tube
Micro Tube
DW
5× PCR Buffer
dNTP　(2.5mM)
Primer(Forward & Reverse)　 (20µM)
Template DNA
PrimeSTAR® HS DNA Polymerase　(2.5U/μl)

Add following components on ice.
- DW
- 5× PCR Buffer
- dNTP　(2.5mM)
- Primer(Forward & Reverse)　 (20µM)
- Template DNA
- PrimeSTAR® HS DNA Polymerase　(2.5U/μl)
Dispense PCR solution to PCR tubes.
Set PCR tubes on thermal cycler
Run PCR

Electrophoresis

Gel
Electrophoresis bath
Parafilm
Micro pipette
TAE Buffer
6× Loading Buffer
DW

Set gel in a gel tank. Pour the TAE Buffer into the gel tank.
- Loading Buffer
- DNA solution
- DW
Mix these components on a Parafilm by pipetting.
Pour the mixture sample into well.
Switch on the power-source and run the gel at 100V for 20min.
Observe the band by exposing ultraviolet radiation

Ethanol precipitation

Centrifuge
Micro Tube
Micro pipette
Aspirator
99.5％Ethanol
3.0M Sodium acetate (pH5.2)
TE Buffer

Add 0.1 volume 3M Sodium acetate to the nucleic acid sample and vortex.
Add 4 µl of Dr. GenTLETM Precipitation Carrier and vortex.
Add 2.5 volumes of ethanol and vortex.
Centrifuge at 12,000 rpm at 4˚C for 15 min.
Discard the supernatant.
Rinse the pellet with 70% ethanol and centrifuge again at 12,000 rpm at 4˚C for 5 min.
Discard the supernatant and dry.
Dissolve the pellet in sterilized water or TE buffer.

Plasmid Extraction

Ice
Micro Tube
Micro pipette
Centrifuge
50mM glucose ; 10mM EDTA ; 25ml Tris-HCl (pH 8.0)
5N NaOH
10％ SDS
3M Potassium Acetate (pH 4.8)

Centrifuge the E-coli pre-culture on 12,000 rpm for 5min, and then discard the supernatant.
Add 100µl of the solution (50ｍM glucose; 10mM EDTA; 25ml Tris-HCl(pH 8.0)), and mix it gently
Add 200µl of the 0.2N NaOH; 1％ SDS, and mix it. Incubate on ice for 5min.
Add 150µl of 3M Potassium Acetate (pH 4.8, 5M Acetic acid; 3M Potassium), and mix it. Incubate #on ice for 5min.
Centrifuge on 12,000 rpm for 5min.
Take supernatant into Microtube.

Digestion

Micro Tube
Micro pipette
Heat Block　or Water bus
Digest Enzyme
10×Buffer　
DW

Add below components into a tube and mix them.
- DNA solution
- DW
- 10× Buffer
- Digest enzyme
Incubate at 37°C, from 2h to 16h

Ligation

Micro Tube
Micro pipette
Heat Block
T4 Ligase
10× Buffer　
DW

Add below components into a tube and mix them.
- DNA solution 1
- DNA solution 2　　　
- DW
- 10× Buffer
- T4 Ligase
Incubate at 16°C, from 30min to 1h

Transformation

Micro pipette
Heat Block　or Water bus
ECOS™ Competent E. coli
Plate (Antibiotic)
Spreader

Keep competent cells on ice to thaw it.
Add plasmid DNA into E.coli cells.
Incubate on ice for 5 min.
Put tubes into water bath at 42℃ for 45 seconds.
Put tubes back on ice for 2 minutes.
Add four times volume of LB (with no antibiotic added). Incubate tubes for 30 min at 37℃.
Spread about 100 ul of the resulting culture on LB plates
Incubate overnight.

Colony PCR(Takara EX® Taq)

Plate
Ice
Micro pipette
Thermal cycler
Burner
70％EtOH
Toothpick
PCRTube
Micro Tube
Spreader
DW
10× PCR Buffer
dNTP (2.5mM)
primer(Forward & Reverse)　(20µM)
Taq Polymerase

Add the all following components on ice.
- DW
- 10× PCR Buffer
- dNTP　(2.5mM)
- Primer(Forward & Reverse)　 (20µM)
- Template DNA
- Taq Polymerase
Dispense PCR solution to PCR tubes.
Pick up a colony and put it into PCR tube.then inoculate to master plate.
Set PCR tubes on thermal cycler
Run PCR

Making Medium for Culture

Erlenmeyer flask
Graduated cylinder
Test Tube or Plate
Autoclave
Stirrer
Electronic balance
Burner or Clean bench
Yeast Extract
Peptone
NaCl
Antibiotic
Agar

Measure component of medium and mix them in Erlenmeyer flask.
Autoclave(121℃,20min).
(Add appropriate antibiotics)
Dispense medium to test tube or plate.
Store at 4℃

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