Team:TMU-Tokyo/Notebook/Protocol/

From 2012.igem.org

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<p class="description">
<p class="description">
<b>■PCR</b><Br></p>
<b>■PCR</b><Br></p>
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<Br>・PCR; PrimeSTAR® HS DNA Polymerase<Br>
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<Br><b>・PCR; PrimeSTAR® HS DNA Polymerase</b><Br>
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<Br>
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1. Add following components on ice.<Br>
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1. Add following components on ice.<Br>
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<div style="margin-left:20px"><p class="description3">
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<Br>
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■General reaction mixture for PCR: 1tube Total 50µL<Br>
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General reaction mixture for PCR (1tube Total 50 μl) <Br>
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(5X PrimeSTAR Buffer 10µL / dNTP Mixture 4µL / Primer(Forward) 0.75µL(20µM) / Primer(Reverse) 0.75µL(20µM) / Template DNA(<i>E. coli</i> Genomic DNA 100 pg - 100 ng plasmidDNA 10 pg - 1 ng) / PrimeSTAR HS DNA Polymerase (2.5 U/µL) 0.5µL / Sterilized distilled water up to 50µL)
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5X PrimeSTAR Buffer 10 μl<Br>
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dNTP Mixture 4 μl<Br>
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2. Dispense PCR solution to PCR tubes.<Br>
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Primer(Forward) 0.75μl(20μM)<Br>
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3. Set PCR tubes on thermal cycler<Br>
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Primerr(Reverse)R 0.75μl(20μM)<Br>
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4. Run PCR<Br>
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Template DNA (E. coli Genomic DNA 100 pg - 100 ng plasmidDNA 10 pg - 1 ng)<Br>
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<div style="margin-left:20px"><p class="description3">
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PrimeSTAR HS DNA Polymerase (2.5 U/μl) 0.5 μl<Br>
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Sterilized distilled water up to 50 μl<Br>
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<Br>
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2. Dispense PCR solution to PCR tubes.<Br>
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3. Set PCR tubes on thermal cycler<Br>
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4. Run PCR<Br>
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   General PCR Conditions <Br>
   General PCR Conditions <Br>
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4℃・・・∞<Br>
4℃・・・∞<Br>
30Cycle  
30Cycle  
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<Br><b>・Colony PCR ; Takara EX®Taq</b><Br>
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1. Add the all following components on ice.
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<Br>・Colony PCR ; Takara EX®Taq <Br>
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1. Add the all following components on ice.
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General reaction mixture for Colony PCR (1tube Total 20 μl)
General reaction mixture for Colony PCR (1tube Total 20 μl)
DW
DW
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& Reverse)0.64  (20µM)
& Reverse)0.64  (20µM)
Taq Polymerase 0.01
Taq Polymerase 0.01
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2. Dispense PCR solution to PCR tubes.
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2. Dispense PCR solution to PCR tubes.
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3. Pick up a colony and put it into PCR tube.then inoculate to master plate.
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3. Pick up a colony and put it into PCR tube.then inoculate to master plate.
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4. Set PCR tubes on thermal cycler
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4. Set PCR tubes on thermal cycler
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5. Run PCR
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5. Run PCR
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5

Revision as of 17:34, 24 September 2012

 




■Experiment
1st week (8.13 - 8.19)
2nd week (8.20 - 8.26)
3rd week (8.27 - 9. 2)
4th week (9. 3 - 9. 9)
5th week (9.10 - 9.16)
6th week (9.17 - 9.23)
7th week (9.24 - 9.30)


■Protocols
Plasmid DNA Purification
Genome DNA Purification
Restruction Enzyme Degestion
DNA Fragment Ligation
Transformation
Electrophoresis
LB Medium


■Assay
Device1 Assay
Device2 Assay
Device3 Assay




Protocol



Our experiment was done follow description.


■Plasmid DNA Purification; (QIAGEN)

All centrifuge is done at 13,000rpm, room temperature.

1. Add 1mL overnight cultures of E. coli in LB medium to a eppendorf tube. Centrifuge 1 min and create pellet.
2. Add 250µL Buffer P1 and vortex until pellet perfectly dissolved.
3. Add 250µL Buffer P2 and mix softly by inverting the tube 4-6 times. (Don't vortex.)
4. Add 350µL Buffer N3 and immediately mix softly by inverting the tube 4-6 times. (Don't vortex.)
5. Centrifuge 10 min. Add supernatant to QIAprep Spin Column by pipetting.
6. Centrifuge 1 min. Discard the flow-through.
7. Add 500µL Buffer PB and centrifuge 1 min. Discard the flow-through.
8. Add 400µL Buffer PE and centrifuge 1 min. Discard the flow-through.
9. Repeat step8.
10. Centrifuge 1 min additionally.
11. Replace the QIAprep Spin Column in a eppendorf tube. Let stand for 1 min.
12. Add 50µL Buffer EB. Let stand for 1 min.
13. Centrifuge 1 min. The flow-through is plasmid DNA solution.


■Genome DNA Purification; Generation™ Capture Column (QIAGEN)


1. Add 200µL overnight cultures of E. coli in LB medium to the Capture Column.
2. Incubate 1 min at room temperature.
3. Add 400µL DNA Purification Solution 1, incubate 1 min at room temperature.
4. Centrifuge 10 s with tabletop centrifuge.
5. Transfer the Capture Column to the Waste Collection Tube.
6. Add 400µL DNA Purification Solution 1, incubate 1 min at room temperature.
7. Centrifuge 10 s with tabletop centrifuge.
8. Add 200µl DNA Elution Solution 2. (Don't incubate.)
9. Centrifuge 10 s with tabletop centrifuge.
10. Transfer the Capture Column to DNA Collection Tube.
11. Add 100µl DNA Elution Solution 2, incuvate 10 min at 99℃ with heat block.
12. Centrifuge 20 s with tabletop centrifuge. Purified DNA will be released to solution.



■Restruction Enzyme Degestion



■DNA Fragment Ligation



■Transformation



■Electrophoresis



■LB Medium



■PCR


・PCR; PrimeSTAR® HS DNA Polymerase
1. Add following components on ice.

■General reaction mixture for PCR: 1tube Total 50µL
(5X PrimeSTAR Buffer 10µL / dNTP Mixture 4µL / Primer(Forward) 0.75µL(20µM) / Primer(Reverse) 0.75µL(20µM) / Template DNA(E. coli Genomic DNA 100 pg - 100 ng plasmidDNA 10 pg - 1 ng) / PrimeSTAR HS DNA Polymerase (2.5 U/µL) 0.5µL / Sterilized distilled water up to 50µL)

2. Dispense PCR solution to PCR tubes.
3. Set PCR tubes on thermal cycler
4. Run PCR

General PCR Conditions
98 ℃・・・5min
98 ℃・・・10sec.
55 ℃・・・5 or 15sec.  TM value≧55…5sec. TM value<55…15sec.
72 ℃・・・1min×1kbp
72 ℃・・・5min
4℃・・・∞
30Cycle


・Colony PCR ; Takara EX®Taq
1. Add the all following components on ice. General reaction mixture for Colony PCR (1tube Total 20 μl) DW 10× PCR Buffer2 dNTP (2.5mM)1.6 Primer(Forward 0.64 & Reverse)0.64  (20µM) Taq Polymerase 0.01 2. Dispense PCR solution to PCR tubes. 3. Pick up a colony and put it into PCR tube.then inoculate to master plate. 4. Set PCR tubes on thermal cycler 5. Run PCR 5 4 1.6 1.6 0.25