Team:Kyoto/Protocols
From 2010.igem.org
Contents |
Making Media
For LB Media:
- Wash a graduated cylinder with MilliQ.
- Add the following to about 180ml of MilliQ in the graduated cylinder:
- Bacto-yeast extract
- 1.0g (0.5% w/v)
- Tryptone
- 2.0g (1.0% w/v)
- NaCl
- 2.0g (1.0% w/v)
- 1N NaOH
- 200µl
- Seal the graduated cylinder by a Parafilm.
- Dissolve the mixture by inverting the graduated cylinder.
- Adjust volume to 200ml by adding more MilliQ.
- Add the media solution to a 200ml Erlenmeyer flask.
- (To prepare solid media, add 2.4g (1.2%) of agar to the flask.)
- Wrap the tops of the flasks with aluminum foil.
- Place a small piece of auto clave tape on one of the flasks.
- Autoclave the media on a liquids.
- Store at room temperature.
- To pour plates, melt the solid media in the microwave, then place flask in water bath to bring media to 50℃.
- Add 200µl of antibiotic:
- Ampicillin
- 100µg/ml
- Kanamycin
- 50µg/ml
- (Add 0.5 - 1.0% Glucose for protein expression.)
Transformation
- Unfreeze conpitent cells on ice.
- Dry a plate by letting the plate upside down and partly open in incubator.
- Add 1 µl DNA solution and 20µl the compitent cells to 1.5ml tube, let stand for 30min on ice.
- If few colony is observed, increase the amount of the compitent cells or DNA, but make the amount of DNA not to get over that of the compitent cells.
- Heatshock for 60s at 42℃.
- Let stand for 2min on ice.
- Cµlture for 1h in precµlture medium (LB or SOC medium), and plate by using spreader.
- (Do not heat spreader too much because e.coli will dead for heat.
Miniprep
- Use QIAprep Spin Miniprep Kit Cat. No. 27104 by QIAGEN
- Pick a single colony from a freshly streaked selective plate and inoculate a culture of about 3ml LB medium containing the appropriate selective antibiotic.
- Incubate at 170rpm for 8h at 37℃ with vigorous shaking.
- Transfer a half of the culture to a tube.
- Harvest the bacterial cells by centrifugation at 14,000 x g for 1min at 4℃. Remove the medium by decanting.
- Transfer the half of the culture to same tube and harvest as same. Remove the medium by pippetting.
- Resuspend pelleted bacterial cells in 250µl Buffer P1 and mix thoroughly by pippeting.
- Add 250µl Buffer P2 and mix thoroughly by inverting the tube gently 4-6 times.
- Add 350µl Buffer N3 and mix immediately and thoroughly by inverting the tube 4-6 times.
- Centrifuge for 10min at 14,000 x g at 4℃.
- Apply the supernatants from step 10 to the QIAprep spin column by pipetting.
- Centrifuge for 10s in a table-top microcentrifuge. Discard the flow-through.
- Wash the QIAprep spin column by adding 0.5ml Buffer PB and centrifuging for 10s in a table-top microcentrifuge. Discard the flow-through.
- Wash QIAprep spin column by adding 0.65ml Buffer PeE and centrifuging fo 10s in a table-top microcentrifuge.
- Discard the flow-through, and centrifuge for and additional 1min to remove residual wash buffer.
- Place the QIAprep column in a clean tube. To elute DNA, add 50µl water to the center of each QIAprep spin column, let stand for 1min, and centrifuge for 1min.
- Discard the QIAprep spin column.
- Measure the concentration of DNA by using eppendorf BioPhotometer plus.
- Restriction Digestion.
- Agarose Gel Electrophoresis for Confirmation.
PCR
Phosphorylation of Primer
- Mix the following.
- 14µl : Primer (over 50pmole/µl [50µM])
- 2µl : 10xProtruding End Kinase Buffer
- 2µl : 10mM rATP (Dilluted "Code No:ATP-111")
- 2µl : T4 Polynucleotide Kinase
- Let stand for 1h at 37℃.
- For 5min at 95℃ (Deactivate T4 Polynucleotide Kinase).
- Store in the freezer.
- Concentration of the phoshorylated primers is estimated at 10pmole/µl [10µM])
Standard PCR
- Dilute template DNA. If the concentration of DNA is 2-100 ng/µL, transfer 1µl to a clean tube and add 99µl Milli-Q.
- Dilute Primer. If the concentration of Primer is XµM, dilute primer X timers and transfer 1µl to a clean tube and add 99µl Milli-Q.
- Make a solution as the below.
- Let stand for 2min at 94℃.
- 25-40 cycles for 10s at 98℃, for 30s at Tm-5℃, and for 1min (1min for 1kb) at 68℃ (Tm is temparature at which primer will dissolve).
- At 15℃ forever.
- Agarose Gel Electrophoresis for confirmation.
Component | Volume | Final Concentration |
---|---|---|
Water | 28µl | |
25mM MgSO4 | 3µl | 1.5mM |
2mM dNTPs | 5µl | 0.2mM |
10xBuffer for KOD plus ver.2 | 5µl | 1x |
Template DNA | 5µl | 1ng << 50ng |
Primer Forward(10µM) | 1.5µl | 0.3µM |
Primer Reverse(10µM) | 1.5µl | 0.3µM |
KOD plus ver.2 | 1µl | 0.02U/µl |
Total | 50µ |
- * If amplification is not succeeded, try at 4.5 or 6.0µl 25mM MgSO4.
Screening PCR
- Make a Mixture (Do on PCR Bench).
- 10x PCR buffer (Boehringer) : 40µl
- 2.5mM dNTP : 8µl
- primer-1 (4pmole/µl) : 20µl
- primer-2 (4pmole/µl) : 20µl
- Taq polymerase (Boehringer) : 1.6µl
- MilliQ : 310µl (to total 400µl)
- Dispense 25µl x 15 tubes.
- Pick a single colony and transfer it to each tubes.
- Suspend the colony.
- Let stand for 10min at 90℃.
- 30 cycles for 30s at 94℃, for 30s 55℃, and for 1min at 72℃.
- Let stand for 4min at 72℃.
- Add 5ml Loading Buffer to the tubes.
- Agalose Gel Electrophoresis for confirmation.
- Negative Control : Use nothing.
- Positive Control : Use a colony that will yield a product with this primers.
Mutagenesis
- (Point mutation, Deletion, Insertion)
- Mix the following.
- 10xBuffer
- 5µl
- 2mmol/l dNTP
- 5µl
- Primer Forward (10pmol/µl)
- 1.5µl
- Primer Reverse (10pmol/µl)
- 1.5µl
- Template Plasmid (50ng/µl)
- 1µl
- KOD plus ver.2
- 1µl
- MilliQ
- 35µl
- Total
- 50µl
- Control: Instead of KOD plus ver.2, add 1µl MilliQ.
- PCR
- Let stand for 2min at 94℃.
- Xcycles (1cycle for 1kb) for 10s at 98℃ and for Ymin (1min for 1kb) at 68℃.
- Hold at 4℃.
- Restriction Digests (DpnI)
- Take 25µl of the solutions into fresh tubes.
- Add 1µl DpnI (10U/µl).
- Let stand for 1h at 37℃.
- Agarose gel electrophoresis, using 5µl of the solution for confirmation.
- Ligation
- Mix the following.
- Sample
- 2µl
- Ligation high
- 5µl
- T4 Polynucleotide Kinase (5U/µl)
- 1µl
- MilliQ
- 7µl
- Total
- 15µl
- Let stand for 1h at 16℃.
- Mix the following.
- Transformation, using 10µl of the solution.
Gel Electrophoresis
- Prepare 200ml of a 1.0% agarose solution:
- Measure 2.0g agarose into a beaker.
- Add 200ml 1xTAE buffer.
- Wrap the top of the beaker with plastic wrap.
- Punch a hole through the wrap with a pipette tip (To let out steam).
- Dissolve the agarose by heating in microwave and swirling without boiling.
- Allow the agarose to cool.
- Pour the agarose solution into a gel tray on a gel maker.
- If there is air bubbles, pushing them with a pipette tip.
- Place comb in the maker.
- Cover the maker with a plastic wrap.
- Let stand for about 45min.
- Remove the comb carefully.
- Store in the Tupperware in the refrigerator.
- Place the tray in electrophoresis chamber.
- Cover the tray with 1xTAE buffer.
- Prepare samples for electrophoresi:
- Add 1µl of 6x Loading Buffer for every 5µl of DNA solution.
- Mix well.
- Load 6µl of the DNA solution per well.
- Electrophorese at 100volts for about 30min until Loading Buffer have migrated approximately three-quaters of the gel.
- Stain the gel in 0.5µg/ml ethidium bromide for 20-30min.
- Rinse the gel with MilliQ.
- Place a plastic wrap on the transilluminator in the cabinet of Printgraph.
- Place the gel on the transilluminator.
- Turn on the transilluminator and confirm the position of the gel.
- Shoot the picture.
- Turn off the transilluminator.
- Dispose of the gel.
Gel Extraction
- Use QIAquick Gel Extraction Kit
- Transfer cutted gel to a tube.
- Add BufferQC about 3 times as much as the volume of the gel.
- Stand the gel for 10 min at 50℃ to Dissolve. If hard to dissolve, sometimes vortex.
- Confirm the color of the solution. If the color is orange or purple, add about 10µl 3M sodium acetate to yellow.
- Add isopropanol as much as the gel and mix.
- Apply the solution to the column.
- Centrifuge for 1 min at 1300 rpm. Discard the flow-through. If the amount of the sample is much, repeat this step by same column.
- Add 500 µl BufferQC and centrifuge for 1 min. Discard the through.
- Add 750 µl BufferPE and let stand for 2-3 min. If the solution overflows, we decrease the amount of BufferPE.
- Centrifuge for 1 min and Discard the through.
- Centrifuge for additional 1 min to remove residual buffer.
- Place the column in a clean tube.
- Add 10 µl BufferEB or H20 to the center of each column, let stand for 1 min, and repeat this step.
- Centrifuge for 1 min at 13000 rpm.
- Discard the column.
Ligation
- Create a Mixture (the vector and the insert at 1 : 5-10 molecµle) and a Control (only the vector).
- Add Ligation High to create a solution.
- Incubate at 16℃ for 30 min.
- If the colonies of E.coli transformed with the Control,