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Team:Tokyo Metropolitan/Project/Pattern/Protocol
From 2010.igem.org
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{{:Team:Tokyo_Metropolitan/Header}} | {{:Team:Tokyo_Metropolitan/Header}} | ||
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| + | <div style="width: 700px; margin-left: 100px; padding-top: 25px; padding-left: 20px;"> | ||
| + | ---- | ||
| + | |||
==PCR with Pho DNA Polymerase (NIPPON GENE)== | ==PCR with Pho DNA Polymerase (NIPPON GENE)== | ||
===<Materials>=== | ===<Materials>=== | ||
| Line 20: | Line 24: | ||
#* dNTP 20μl (starting with 2.5mM) <br /> | #* dNTP 20μl (starting with 2.5mM) <br /> | ||
#* DW 85µl<br /> | #* DW 85µl<br /> | ||
| - | # | + | #* '''Total reaction Mix 125μl'''<br /> |
# Add all components together, except for the template. Mix thoroughly by inversion. Spin down. <br /> | # Add all components together, except for the template. Mix thoroughly by inversion. Spin down. <br /> | ||
# Add the template DNA(pellet or Plasmid) for your samples in to PCR tubes<br /> | # Add the template DNA(pellet or Plasmid) for your samples in to PCR tubes<br /> | ||
| Line 33: | Line 37: | ||
| + | |||
| + | |||
| + | ---- | ||
==PCR with Tag DNA Polymerase (NIPPON GENE)== | ==PCR with Tag DNA Polymerase (NIPPON GENE)== | ||
| Line 45: | Line 52: | ||
===<Process>=== | ===<Process>=== | ||
| - | + | # Make the pellet with pre-culture<br /> | |
| - | + | # Thaw all required reagents completely and put them on ice. Mix all reagents well by inversion and spin them down prior to pipeting. <br /> | |
| - | + | # Prepare the reaction mix to correct for dispensing losses prepare an excess of reaction mix (for example, a 100 reactions mix for 96 reactions) <br /> | |
| - | + | #* 10x reaction buffer 12.5μl<br /> | |
| - | + | #* Forward primer 2.5μl (starting with 20µM) <br /> | |
| - | + | #* Reverse primer 2.5μl (starting with 20µM) <br /> | |
| - | + | #* Tag DNA Polymerase 1.0µl (starting with 2.5U/µl) <br /> | |
| - | + | #* dNTP 10μl (starting with 2.5mM) <br /> | |
| - | + | #* DW 96.5µl<br /> | |
| - | + | #* '''Total reaction Mix 125μl'''<br /> | |
| - | + | # Add all components together, except for the template. Mix thoroughly by inversion. Spin down. <br /> | |
| - | + | # Add the template DNA(pellet or Plasmid) for your samples in to PCR tubes<br /> | |
| - | + | # Add 50μl of the reaction mix per tube and mix gently on a stirrer or spin down. Ensure that no bubbles are present in the reaction tube. Reaction set up can be done at room temperature. <br /> | |
| - | + | # Program your Real-Time Thermocycler w/ “fast block” using the following recommended FAST parameters: <br /> | |
| - | + | #* 95°C 5min. <br /> | |
| - | + | #* 95°C 30sec. 30cycle<br /> | |
| - | + | #* 55°C 30sec. 30cycle<br /> | |
| - | + | #* Tm-5°C 2~4min. 30cycle<br /> | |
| - | + | #* 72°C 5min. <br /> | |
| - | + | #* 4°C ∞<br /> | |
| + | |||
| + | |||
| + | ---- | ||
==DNA Ligation with Ligation-convenience kit (NIPPON GENE)== | ==DNA Ligation with Ligation-convenience kit (NIPPON GENE)== | ||
| - | <Materials> | + | ===<Materials>=== |
| - | + | * DNA solution<br /> | |
| - | + | * 2 × Ligation Mix (Ligation-convenience kit from NIPPON GENE) <br /> | |
| - | < | + | ===<Process>=== |
| - | + | # Prepare 10 μl of DNA solution to contain DNA fragment with appropriate mole ratio against vector DNA. <br /> | |
| - | + | # Add 10μl of 2 × Ligation Mix to the DNA solution and mix well. <br /> | |
| - | + | # Ligation reaction. Incubate 5-30min at 16°C. <br /> | |
| - | + | # Apply DNA reaction mixture directly to transformation or in vitro packaging as it is. <br /> | |
| + | |||
| + | |||
| + | ---- | ||
==DNA extraction== | ==DNA extraction== | ||
| - | <Materials> | + | ===<Materials>=== |
| - | + | * Binding Buffer (5M Guanidine Thiocyanate; 100mM Tris-HCl (pH7.0))<br /> | |
| - | + | * Wash Buffer (10mM Tris-HCl (pH7.5))<br /> | |
| - | + | * Silica gel solution<br /> | |
| - | + | * TE (10mM Tris-HCl pH 8.0; 0.1mM EDTA)<br /> | |
| - | + | * Sample<br /> | |
| - | + | ===<Process>=== | |
| - | + | # Add 150µl of Binding Buffer to the tube and Vortex. <br /> | |
| - | + | # Add 10µl of Silica gel solution to the tube and Vortex.<br /> | |
| - | + | # Vortex every 1min for 5min.<br /> | |
| - | + | # Centrifuge on 12,000 rpm for 1min, and then aspirate the supernatant. <br /> | |
| - | + | # Add 200µl of Wash Buffer to tube and Vortex.<br /> | |
| - | + | # Centrifuge on 12,000 rpm for 30sec, and then aspirate the supernatant. <br /> | |
| - | + | # Add 200µl of Wash Buffer to tube and Vortex.<br /> | |
| - | + | # Centrifuge on 12,000 rpm for 30sec, and then aspirate the supernatant. <br /> | |
| - | + | # Dry the pellets in the speed-vac for 5min, or air dry.<br /> | |
| - | + | # Add 20µl of TE Buffer to the dried pellets<br /> | |
| + | |||
| + | ---- | ||
==DNA extraction with ISOPLANT(NIPPON GENE)== | ==DNA extraction with ISOPLANT(NIPPON GENE)== | ||
| - | <Materials> | + | ===<Materials>=== |
| - | + | * Extraction Buffer<br /> | |
| - | + | * Lysis Bufferl<br /> | |
| - | + | * Sodium Acetate(pH5.2)<br /> | |
| - | + | * 10mM Tris-HCl(pH8.0), 1mM EDTA<br /> | |
| - | + | * 1mg/ml RNaseA<br /> | |
| - | + | * E-coli culture<br /> | |
| - | + | * TE(10mM Tris-HCl pH 8.0; 0.1mM EDTA)<br /> | |
| - | + | * DW<br /> | |
| + | ===<Process>=== | ||
| + | # Centrifuge 1.5ml of E-coli culture at 4οC for 5min, and then aspirate the supernatant. <br /> | ||
| + | # Add 0.3ml of Extraction Buffer to sample, and then vortex 1~2sec. <br /> | ||
| + | # Add 0.15mlof Lysis Buffer to solution, and then vortex 5~6sec. <br /> | ||
| + | # Incubate 15min at 50°C. <br /> | ||
| + | # Add 0.15ml of Sodium Acetate(pH5.2) to solution, and then vortex 1~2sec. <br /> | ||
| + | # Leave on ice for 15min.<br /> | ||
| + | # Centrifuge solution at 4οC for 15min, and then aspirate the supernatant. <br /> | ||
| + | # Add 0.3ml of H2O to the tube having the pellets, and then vortex thoroughly. <br /> | ||
| + | # Add 0.6ml of EtOH to solution, and then vortex thoroughly. <br /> | ||
| + | # Centrifuge solution for 10min, and then aspirate the supernatant. <br /> | ||
| + | # Add 70%EtOH to the tube having the pellets. <br /> | ||
| + | # Dry the pellets in the speed-vac for 5min, or air dry.<br /> | ||
| + | # Add TE Buffer to the dried pellets<br /> | ||
| - | |||
| - | |||
| - | |||
| - | |||
| - | |||
| - | |||
| - | |||
| - | |||
| - | |||
| - | |||
| - | |||
| - | |||
| - | |||
| - | |||
| + | ---- | ||
| + | ==Plasmid extraction from E-coli== | ||
| + | ===<Materials>=== | ||
| + | * Binding Buffer (5M Guanidine Thiocyanate; 100mM Tris-HCl (pH7.0))<br /> | ||
| + | * Wash Buffer (10mM Tris-HCl (pH7.5))<br /> | ||
| + | * Silica gel solution<br /> | ||
| + | * TE (10mM Tris-HCl pH 8.0; 0.1mM EDTA)<br /> | ||
| + | * Sample<br /> | ||
| + | ===<Process>=== | ||
| + | # Centrifuge 1ml of the E-coli pre-culture on 12,000 rpm for 30sec, and then aspirate the supernatant. <br /> | ||
| + | # Add 100µl of the solution (50mM glucose; 10mM EDTA; 25ml Tris-HCl(pH 8.0)), and mix it gently<br /> | ||
| + | # Add 200µl of the 0.2N NaOH; 1% SDS, and mix it, and then incubate on ice for 5min.<br /> | ||
| + | # Add 150µl of 3M Potassium Acetate (pH 4.8)(5M Acetic acid; 3M Potassium), and mix it, and then incubate on ice for 5min.<br /> | ||
| + | # Centrifuge on 12,000 rpm for 5min.<br /> | ||
| + | # Add 400µl of Binding Buffer and 10µl of Silica gel solution to another tube and Vortex. <br /> | ||
| + | # Add the supernatant(in centrifuged tube) to solution of Binding Buffer and Silica gel, and Vortex.<br /> | ||
| + | # Centrifuge on 12,000 rpm for 5min, and then aspirate the supernatant. <br /> | ||
| + | # Add 800µl of Wash Buffer to tube and Vortex.<br /> | ||
| + | # Centrifuge on 12,000 rpm for 30sec, and then aspirate the supernatant. <br /> | ||
| + | # Add 800µl of Wash Buffer to tube and Vortex.<br /> | ||
| + | # Centrifuge on 12,000 rpm for 30sec, and then aspirate the supernatant. <br /> | ||
| + | # Dry the pellets in the speed-vac for 5min, or air dry.<br /> | ||
| + | # Add 50µl of TE Buffer to the dried pellets<br /> | ||
| - | |||
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| - | |||
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| - | |||
| - | |||
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| - | |||
| - | |||
| - | |||
| - | |||
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| - | |||
| - | |||
| - | |||
| - | |||
| - | |||
| - | |||
| - | |||
| + | ---- | ||
| + | ==Transformation with ECOS competent E-coli(NIPPON GENE)== | ||
| + | ===<Materials>=== | ||
| + | * competent cell<br /> | ||
| + | * Plasmid solution<br /> | ||
| + | * LB plate(Amp)<br /> | ||
| - | == | + | ===<Process>=== |
| - | + | # Keep a competent cell(JM109) at RT and then on ice until melting.<br /> | |
| - | + | # Add 5µl of the solution of ligated-recombinant plasmid DNA to the tube, which contains the competent cell, and mix it gently.<br /> | |
| - | . | + | # Keep the tube on ice for 5min.<br /> |
| - | . | + | # Transfer the tube into 42°C water bath and keep it for 45sec.<br /> |
| + | # Vortex a suspension and spread it on a LB plate.<br /> | ||
| + | # Incubate the plate at 37°C for 12~16h.<br /> | ||
| - | |||
| - | |||
| - | |||
| - | |||
| - | |||
| - | |||
| - | |||
| + | |||
| + | ---- | ||
==Electrophoresis== | ==Electrophoresis== | ||
| - | <Materials> | + | ===<Materials>=== |
| - | + | * TAE Buffer 100ml<br /> | |
| - | + | * Agarose 1.0g<br /> | |
| - | + | * Marker 5.0µl<br /> | |
| - | + | * Dye 1.0µl<br /> | |
| - | + | * DNA solution<br /> | |
| - | + | ===<Process>=== | |
| - | + | # TAE Buffrer into agarose and Microwave for about 1min to dissolve the agarose. <br /> | |
| - | + | # Pour the agarose slowly into the gel board. <br /> | |
| - | + | # Set gel in a gel tank. <br /> | |
| - | + | # Pour the TAE Buffer into the gel tank. <br /> | |
| - | + | # Mix the marker, DW and Dye. <br /> | |
| - | + | # Pour the mixture sample into well. <br /> | |
| - | + | # Close the gel tank, switch on the power-source and run the gel at 100V for 20min. <br /> | |
| - | + | # Switch off and unplug the gel tank and carry the gel to the machine to look at the progress of the gel. <br /> | |
| + | ===<Marker>=== | ||
| + | One of the marker we used is "OneSTEP Ladder 50"[http://www.nippongene.com/index/english/e_index.htm/ (NIPPONE GENE)] | ||
| + | |||
| + | [[Image:Lad050.png|300x300px|]] | ||
| + | |||
| + | ---- | ||
==DNA Digestion== | ==DNA Digestion== | ||
| - | <Material> | + | ===<Material>=== |
| - | + | * DNA solution<br /> | |
| - | + | * Digest enzyme<br /> | |
| - | + | * ×10 Buffer<br /> | |
| - | + | * DW<br /> | |
| - | + | ===<Process>=== | |
| - | + | # Add 5µl of DW and 2µl of ×10 Buffer into the tube, and mix it gently.<br /> | |
| - | + | # Add 10µl of DNA solution and 1µl of Digest enzyme into the tube, and mix it gently.<br /> | |
| - | + | # Incubate at 37°C for 5h.<br /> | |
| - | |||
| - | |||
| - | |||
| + | ---- | ||
| - | + | ==Ligation with Ligation-convenience kit (NIPPON GENE)== | |
| + | ===<Materials>=== | ||
| + | *DNA solution | ||
| + | * 2×Ligation Mix (Ligation-convenience kit NIPPON GENE) | ||
| + | ===<Process>=== | ||
| + | #Prepare 10 μl of DNA solution to contain DNA fragment with appropriate mole ratio against vector DNA. | ||
| + | #Add 10μl of 2 × Ligation Mix to the DNA solution and mix well. | ||
| + | # Ligation reaction. Incubate 5-30min at 16°C. | ||
| + | #Apply DNA reaction mixture directly to transformation or in vitro packaging as it is. | ||
| - | |||
| - | |||
| - | |||
| - | |||
| - | |||
| + | ---- | ||
| + | ==DNA extraction with ISOPLANT(NIPPON GENE)== | ||
| + | ===<Materials>=== | ||
| + | *Extraction Buffer 0.3ml | ||
| + | *Lysis Buffer 0.15ml | ||
| + | *Sodium Acetate(pH5.2) 0.15ml | ||
| + | *10mM Tris-HCl(pH8.0), 1mM EDTA 0.1ml | ||
| + | *1mg/ml RNaseA 1µl | ||
| + | *E-coli culture | ||
| + | *H20 | ||
| + | *TE Buffer | ||
| + | ===<Process>=== | ||
| + | # Centrifuge 1.5ml of E-coli culture at 4οC for 5min, and then aspirate the supernatant. | ||
| + | # Add 0.3ml of Extraction Buffer to sample, and then vortex 1~2sec. | ||
| + | # Add 0.15mlof Lysis Buffer to solution, and then vortex 5~6sec. | ||
| + | # Incubate 15min at 50°C. | ||
| + | # Add 0.15ml of Sodium Acetate(pH5.2) to solution, and then vortex 1~2sec. | ||
| + | # Leave on ice for 15min | ||
| + | # Centrifuge solution at 4οC for 15min, and then aspirate the supernatant. | ||
| + | # Add 0.3ml of H2O to the tube having the pellets, and then vortex thoroughly. | ||
| + | # Add 0.6ml of EtOH to solution, and then vortex thoroughly. | ||
| + | # Centrifuge solution for 10min, and then aspirate the supernatant. | ||
| + | # Add 70%EtOH to the tube having the pellets. | ||
| + | # Dry the pellets in the speed-vac for 5min, or air dry. | ||
| + | # Add TE Buffer to the dried pellets | ||
| - | == | + | |
| - | + | ||
| - | + | ---- | |
| - | + | ||
| - | + | ==About Sample== | |
| - | + | ||
| - | + | <table border="1" align="center"> | |
| - | E | + | <TR><TD> No. </TD><TD>template</TD><TD>'''fragment'''<TD>Digest enzyme</TD><TD>bp<TR> |
| - | + | <TR><TD> 1 </TD><TD>BBa_K208017</TD><TD>'''Promoter-signal'''</TD><TD>AvrⅡ</TD><TD>266<TR> | |
| - | + | <TR><TD> 2 </TD><TD>E.coli genome</TD><TD>'''CyaA'''</TD><TD>NheⅠ</TD><TD>2583<TR> | |
| - | + | <TR><TD> 3 </TD><TD>BBa_l12521</TD><TD>'''mRFP1-terminator'''</TD><TD>NheⅠ</TD><TD>861<TR> | |
| - | + | <TR><TD> 4 </TD><TD>BBa_K208017</TD><TD>'''Promoter'''</TD><TD>AvrⅡ</TD><TD>145<TR> | |
| - | + | <TR><TD> 5 </TD><TD>BBa_K208017</TD><TD>'''RBS-signal'''</TD><TD>SpeⅠ</TD><TD>103<TR> | |
| - | + | <TR><TD> 6 </TD><TD>BBa_l732901</TD><TD>'''LacZ'''</TD><TD>SpeⅠ</TD><TD>3093<TR> | |
| - | 4 | + | <TR><TD> 7 </TD><TD>BBa_l12521</TD><TD>'''terminator'''</TD><TD>NheⅠ</TD><TD>167<TR> |
| - | 5 | + | <TR><TD> 8 </TD><TD>E. coli genome</TD><TD>'''CRP'''</TD><TD>AvrⅡ</TD><TD>657<TR> |
| - | 6 | + | <TR><TD> 9 </TD><TD>BBa_K156010</TD><TD>'''SBFP2'''</TD><TD>XbaⅠ</TD><TD>721<TR> |
| - | 7 | + | <TR><TD> 10 </TD><TD>BBa_J23110</TD><TD>'''Promoter-RBS'''</TD><TD>SpeⅠ</TD><TD>70<TR> |
| - | 8 | + | </table> |
| - | 9 | + | |
| - | 10 | + | |
| - | + | ||
| - | + | ||
| - | + | ||
Latest revision as of 10:03, 27 October 2010
PCR with Pho DNA Polymerase (NIPPON GENE)
<Materials>
- 10x reaction buffer
- Forward primer (starting with 20µM)
- Reverse primer (starting with 20µM)
- Pho DNA Polymerase (starting with 2.5U/µl)
- dNTP (starting with 2.5mM)
- DW
- DNA samples
<Process>
- Make the pellet with pre-colony
- Thaw all required reagents completely and put them on ice. Mix all reagents well by inversion and spin them down prior to pipeting.
- Prepare the reaction mix to correct for dispensing losses prepare an excess of reaction mix (for example, a 100 reactions mix for 96 reactions)
- 10x reaction buffer 12.5μl
- Forward primer 2.5μl (starting with 20µM)
- Reverse primer 2.5μl (starting with 20µM)
- Pho DNA Polymerase 2.5µl (starting with 2.5U/µl)
- dNTP 20μl (starting with 2.5mM)
- DW 85µl
- Total reaction Mix 125μl
- 10x reaction buffer 12.5μl
- Add all components together, except for the template. Mix thoroughly by inversion. Spin down.
- Add the template DNA(pellet or Plasmid) for your samples in to PCR tubes
- Add 50μl of the reaction mix per tube and mix gently on a stirrer or spin down. Ensure that no bubbles are present in the reaction tube. Reaction set up can be done at room temperature.
- Program your Real-Time Thermocycler w/ “fast block” using the following recommended FAST parameters:
- 95°C 5min.
- 95°C 30sec. 30cycle
- 55°C 30sec. 30cycle
- Tm-5°C 2~4min. 30cycle
- 72°C 5min.
- 4°C ∞
- 95°C 5min.
PCR with Tag DNA Polymerase (NIPPON GENE)
<Materials>
- 10x reaction buffer
- Forward primer (starting with 20µM)
- Reverse primer (starting with 20µM)
- Tag DNA Polymerase (starting with 2.5U/µl)
- dNTP (starting with 2.5mM)
- DW
- DNA samples
<Process>
- Make the pellet with pre-culture
- Thaw all required reagents completely and put them on ice. Mix all reagents well by inversion and spin them down prior to pipeting.
- Prepare the reaction mix to correct for dispensing losses prepare an excess of reaction mix (for example, a 100 reactions mix for 96 reactions)
- 10x reaction buffer 12.5μl
- Forward primer 2.5μl (starting with 20µM)
- Reverse primer 2.5μl (starting with 20µM)
- Tag DNA Polymerase 1.0µl (starting with 2.5U/µl)
- dNTP 10μl (starting with 2.5mM)
- DW 96.5µl
- Total reaction Mix 125μl
- 10x reaction buffer 12.5μl
- Add all components together, except for the template. Mix thoroughly by inversion. Spin down.
- Add the template DNA(pellet or Plasmid) for your samples in to PCR tubes
- Add 50μl of the reaction mix per tube and mix gently on a stirrer or spin down. Ensure that no bubbles are present in the reaction tube. Reaction set up can be done at room temperature.
- Program your Real-Time Thermocycler w/ “fast block” using the following recommended FAST parameters:
- 95°C 5min.
- 95°C 30sec. 30cycle
- 55°C 30sec. 30cycle
- Tm-5°C 2~4min. 30cycle
- 72°C 5min.
- 4°C ∞
- 95°C 5min.
DNA Ligation with Ligation-convenience kit (NIPPON GENE)
<Materials>
- DNA solution
- 2 × Ligation Mix (Ligation-convenience kit from NIPPON GENE)
<Process>
- Prepare 10 μl of DNA solution to contain DNA fragment with appropriate mole ratio against vector DNA.
- Add 10μl of 2 × Ligation Mix to the DNA solution and mix well.
- Ligation reaction. Incubate 5-30min at 16°C.
- Apply DNA reaction mixture directly to transformation or in vitro packaging as it is.
DNA extraction
<Materials>
- Binding Buffer (5M Guanidine Thiocyanate; 100mM Tris-HCl (pH7.0))
- Wash Buffer (10mM Tris-HCl (pH7.5))
- Silica gel solution
- TE (10mM Tris-HCl pH 8.0; 0.1mM EDTA)
- Sample
<Process>
- Add 150µl of Binding Buffer to the tube and Vortex.
- Add 10µl of Silica gel solution to the tube and Vortex.
- Vortex every 1min for 5min.
- Centrifuge on 12,000 rpm for 1min, and then aspirate the supernatant.
- Add 200µl of Wash Buffer to tube and Vortex.
- Centrifuge on 12,000 rpm for 30sec, and then aspirate the supernatant.
- Add 200µl of Wash Buffer to tube and Vortex.
- Centrifuge on 12,000 rpm for 30sec, and then aspirate the supernatant.
- Dry the pellets in the speed-vac for 5min, or air dry.
- Add 20µl of TE Buffer to the dried pellets
DNA extraction with ISOPLANT(NIPPON GENE)
<Materials>
- Extraction Buffer
- Lysis Bufferl
- Sodium Acetate(pH5.2)
- 10mM Tris-HCl(pH8.0), 1mM EDTA
- 1mg/ml RNaseA
- E-coli culture
- TE(10mM Tris-HCl pH 8.0; 0.1mM EDTA)
- DW
<Process>
- Centrifuge 1.5ml of E-coli culture at 4οC for 5min, and then aspirate the supernatant.
- Add 0.3ml of Extraction Buffer to sample, and then vortex 1~2sec.
- Add 0.15mlof Lysis Buffer to solution, and then vortex 5~6sec.
- Incubate 15min at 50°C.
- Add 0.15ml of Sodium Acetate(pH5.2) to solution, and then vortex 1~2sec.
- Leave on ice for 15min.
- Centrifuge solution at 4οC for 15min, and then aspirate the supernatant.
- Add 0.3ml of H2O to the tube having the pellets, and then vortex thoroughly.
- Add 0.6ml of EtOH to solution, and then vortex thoroughly.
- Centrifuge solution for 10min, and then aspirate the supernatant.
- Add 70%EtOH to the tube having the pellets.
- Dry the pellets in the speed-vac for 5min, or air dry.
- Add TE Buffer to the dried pellets
Plasmid extraction from E-coli
<Materials>
- Binding Buffer (5M Guanidine Thiocyanate; 100mM Tris-HCl (pH7.0))
- Wash Buffer (10mM Tris-HCl (pH7.5))
- Silica gel solution
- TE (10mM Tris-HCl pH 8.0; 0.1mM EDTA)
- Sample
<Process>
- Centrifuge 1ml of the E-coli pre-culture on 12,000 rpm for 30sec, and then aspirate 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, and then incubate on ice for 5min.
- Add 150µl of 3M Potassium Acetate (pH 4.8)(5M Acetic acid; 3M Potassium), and mix it, and then incubate on ice for 5min.
- Centrifuge on 12,000 rpm for 5min.
- Add 400µl of Binding Buffer and 10µl of Silica gel solution to another tube and Vortex.
- Add the supernatant(in centrifuged tube) to solution of Binding Buffer and Silica gel, and Vortex.
- Centrifuge on 12,000 rpm for 5min, and then aspirate the supernatant.
- Add 800µl of Wash Buffer to tube and Vortex.
- Centrifuge on 12,000 rpm for 30sec, and then aspirate the supernatant.
- Add 800µl of Wash Buffer to tube and Vortex.
- Centrifuge on 12,000 rpm for 30sec, and then aspirate the supernatant.
- Dry the pellets in the speed-vac for 5min, or air dry.
- Add 50µl of TE Buffer to the dried pellets
Transformation with ECOS competent E-coli(NIPPON GENE)
<Materials>
- competent cell
- Plasmid solution
- LB plate(Amp)
<Process>
- Keep a competent cell(JM109) at RT and then on ice until melting.
- Add 5µl of the solution of ligated-recombinant plasmid DNA to the tube, which contains the competent cell, and mix it gently.
- Keep the tube on ice for 5min.
- Transfer the tube into 42°C water bath and keep it for 45sec.
- Vortex a suspension and spread it on a LB plate.
- Incubate the plate at 37°C for 12~16h.
Electrophoresis
<Materials>
- TAE Buffer 100ml
- Agarose 1.0g
- Marker 5.0µl
- Dye 1.0µl
- DNA solution
<Process>
- TAE Buffrer into agarose and Microwave for about 1min to dissolve the agarose.
- Pour the agarose slowly into the gel board.
- Set gel in a gel tank.
- Pour the TAE Buffer into the gel tank.
- Mix the marker, DW and Dye.
- Pour the mixture sample into well.
- Close the gel tank, switch on the power-source and run the gel at 100V for 20min.
- Switch off and unplug the gel tank and carry the gel to the machine to look at the progress of the gel.
<Marker>
One of the marker we used is "OneSTEP Ladder 50"[http://www.nippongene.com/index/english/e_index.htm/ (NIPPONE GENE)]
DNA Digestion
<Material>
- DNA solution
- Digest enzyme
- ×10 Buffer
- DW
<Process>
- Add 5µl of DW and 2µl of ×10 Buffer into the tube, and mix it gently.
- Add 10µl of DNA solution and 1µl of Digest enzyme into the tube, and mix it gently.
- Incubate at 37°C for 5h.
Ligation with Ligation-convenience kit (NIPPON GENE)
<Materials>
- DNA solution
- 2×Ligation Mix (Ligation-convenience kit NIPPON GENE)
<Process>
- Prepare 10 μl of DNA solution to contain DNA fragment with appropriate mole ratio against vector DNA.
- Add 10μl of 2 × Ligation Mix to the DNA solution and mix well.
- Ligation reaction. Incubate 5-30min at 16°C.
- Apply DNA reaction mixture directly to transformation or in vitro packaging as it is.
DNA extraction with ISOPLANT(NIPPON GENE)
<Materials>
- Extraction Buffer 0.3ml
- Lysis Buffer 0.15ml
- Sodium Acetate(pH5.2) 0.15ml
- 10mM Tris-HCl(pH8.0), 1mM EDTA 0.1ml
- 1mg/ml RNaseA 1µl
- E-coli culture
- H20
- TE Buffer
<Process>
- Centrifuge 1.5ml of E-coli culture at 4οC for 5min, and then aspirate the supernatant.
- Add 0.3ml of Extraction Buffer to sample, and then vortex 1~2sec.
- Add 0.15mlof Lysis Buffer to solution, and then vortex 5~6sec.
- Incubate 15min at 50°C.
- Add 0.15ml of Sodium Acetate(pH5.2) to solution, and then vortex 1~2sec.
- Leave on ice for 15min
- Centrifuge solution at 4οC for 15min, and then aspirate the supernatant.
- Add 0.3ml of H2O to the tube having the pellets, and then vortex thoroughly.
- Add 0.6ml of EtOH to solution, and then vortex thoroughly.
- Centrifuge solution for 10min, and then aspirate the supernatant.
- Add 70%EtOH to the tube having the pellets.
- Dry the pellets in the speed-vac for 5min, or air dry.
- Add TE Buffer to the dried pellets
About Sample
| No. | template | fragment | Digest enzyme | bp |
| 1 | BBa_K208017 | Promoter-signal | AvrⅡ | 266 |
| 2 | E.coli genome | CyaA | NheⅠ | 2583 |
| 3 | BBa_l12521 | mRFP1-terminator | NheⅠ | 861 |
| 4 | BBa_K208017 | Promoter | AvrⅡ | 145 |
| 5 | BBa_K208017 | RBS-signal | SpeⅠ | 103 |
| 6 | BBa_l732901 | LacZ | SpeⅠ | 3093 |
| 7 | BBa_l12521 | terminator | NheⅠ | 167 |
| 8 | E. coli genome | CRP | AvrⅡ | 657 |
| 9 | BBa_K156010 | SBFP2 | XbaⅠ | 721 |
| 10 | BBa_J23110 | Promoter-RBS | SpeⅠ | 70 |
