Team:KAIST Korea/Notebook Protocol
From 2012.igem.org
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<h3>Procedure</h3></br> | <h3>Procedure</h3></br> | ||
- | <h4>Pellet Cells</h4> | + | <h4>1) Pellet Cells</h4> |
<ol> | <ol> | ||
<li>Add 1ml of an overnight culture to a 1.5ml microcentrifuge tube.</li> | <li>Add 1ml of an overnight culture to a 1.5ml microcentrifuge tube.</li> | ||
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</ol> | </ol> | ||
</br> | </br> | ||
- | <h4>Lyse Cells</h4> | + | <h4>2) Lyse Cells</h4> |
<ol start="4"> | <ol start="4"> | ||
<li>Add 1ml of an overnight culture to a 1.5ml microcentrifuge tube.</li> | <li>Add 1ml of an overnight culture to a 1.5ml microcentrifuge tube.</li> | ||
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</ol> | </ol> | ||
</br> | </br> | ||
- | <h4>Protein Precipitation</h4> | + | <h4>3) Protein Precipitation</h4> |
<ol start="7"> | <ol start="7"> | ||
<li>Add 200ul of Protein Precipitation Solution to the RNase-treated cell lysate. Vortex vigorously at high speed for 20seconds to mix the Protein Precipitation Solution tieh the cell lysate.</li> | <li>Add 200ul of Protein Precipitation Solution to the RNase-treated cell lysate. Vortex vigorously at high speed for 20seconds to mix the Protein Precipitation Solution tieh the cell lysate.</li> | ||
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</ol> | </ol> | ||
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<img id="figure" alt="TE buffer" src="https://static.igem.org/mediawiki/2012/d/df/KAIST_Protocol2_table2.png"></img> | <img id="figure" alt="TE buffer" src="https://static.igem.org/mediawiki/2012/d/df/KAIST_Protocol2_table2.png"></img> | ||
<div style="clear:both;"></div> | <div style="clear:both;"></div> | ||
+ | </div> | ||
</div> | </div> | ||
<img src="https://static.igem.org/mediawiki/2012/8/85/Protocol_content_bottom.png" id="bot-part"/> | <img src="https://static.igem.org/mediawiki/2012/8/85/Protocol_content_bottom.png" id="bot-part"/> | ||
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- | <div class="accordionButton"><div id="protocol"> | + | <div class="accordionButton"><div id="protocol">10. SDS PAGE</div></div> |
<div class="accordionContent"> | <div class="accordionContent"> | ||
<img src="https://static.igem.org/mediawiki/2012/7/77/KAIST_Protocol_content_top.png" id="top-part"/> | <img src="https://static.igem.org/mediawiki/2012/7/77/KAIST_Protocol_content_top.png" id="top-part"/> | ||
<div id="protocolcontent"> | <div id="protocolcontent"> | ||
+ | We did sodium dodecyl sulfate polyacrylamide gel electrophoresis according to cold spring harbor protocol.</br></br> <a href="http://cshprotocols.cshlp.org/content/2006/1/pdb.prot4313.full">▶▶Click here to show 'cold spring harbor protocol'</a> | ||
</div> | </div> | ||
<img src="https://static.igem.org/mediawiki/2012/8/85/Protocol_content_bottom.png" id="bot-part"/> | <img src="https://static.igem.org/mediawiki/2012/8/85/Protocol_content_bottom.png" id="bot-part"/> |
Revision as of 17:35, 25 September 2012
2012 KAIST Korea
Mail : kaist.igem.2012@gmail.com
Twitter : twitter.com/KAIST_iGEM_2012
Facebook : www.facebook.com/KAISTiGEM2012
image description
Lab Protocols
Please enter sub title1. LB agar plate
Materials
Procedure
- Add 25g LB broth and 15g agar into 1L DDW.
- Autoclave
2. Genomic DNA Purification
Materials
Procedure
1) Pellet Cells
- Add 1ml of an overnight culture to a 1.5ml microcentrifuge tube.
- Centrifuge at 13000 rpm for 2.5minutes to pellet the cells.
- Remove the supernatant.
2) Lyse Cells
- Add 1ml of an overnight culture to a 1.5ml microcentrifuge tube.
- Centrifuge at 13000 rpm for 2.5minutes to pellet the cells.
- Remove the supernatant.
3) Protein Precipitation
- Add 200ul of Protein Precipitation Solution to the RNase-treated cell lysate. Vortex vigorously at high speed for 20seconds to mix the Protein Precipitation Solution tieh the cell lysate.
- Incubate the sample on ice for 5minutes.
- Centrifuge at 13,000rpm 3minutes.
- Transfer the supernatant containing the DNA to a clean 1.5ml microcentrifuge tube. Note: Some supernatant may remain in the original tube containing the protein pellet. Leave this residual liquid in the tube to avoid contaminating the DNA solution with the precipitated protein.
- Add 600ul isopropanol.
- Gently mix by inversion until the thread-like strands of DNA form a visible mass.
- Centrifuge at 13000rpm for 2minutes.
- Carefully pour off the supernatant.
- Add 600ul of room temperature 70% ethanol and gently invert the tube 5 times to wash the DNA pellet.
- Centrifuge at 13000rpm for 2minutes. Carefully aspirate the ethanol.
- Drain the tube on clean absorbent paper and allow the pellet to air-dry for 10-14minutes.
- Add 50~100 μl TE buffer and rehydrate the DNA by incubating at 65℃ for 20min. Periodically mix the solution by gently tapping the tube. Alternatively, rehydrate the DNA by incubationg the solution overnight at room temperature or at 4℃.
3. Vector transformation
Procedure
1) Restriction enzyme digestion
- Incubate 2hr at 37℃.
- Inactivation 20min at 65℃.
2) Dephosphorylation (Only for vector)
- Incubate 30min at 37℃.
- Inactivation 5min at 70℃.
3) Ligation
- Incubate 16hr at 16℃.
4) Transformation
- Add 20ul ligated vector into 100ul of competent cell.
- Incubate ice 5min.
- Heat shock 42℃, 1min 30sec.
- Ice 5min.
- Recovery with 700ul LB at 37℃, 1hr.
- Plating.
4. PCR
Procedure
Reaction Conditions
- 95℃ 3min
- 95℃ 30sec
- 54℃ 30sec
- 72℃ 1min/kbp
- 72℃ 10min
- 12℃ ∞
5. Gel extraction
Materials
- MGTM Gel Extraction SV - Macrogen
Procedure
- Excise the DNA band of interest using an ethanol-cleaned razor blade.
- Weigh the gel slice in a microcentrifuge tube. Add 3 volumes (ul) of Buffer GB to 1 volume (mg) of gel.
- Incubate at 50°C until the agarose gel is completely melted (5 ~ 10 min).
- Transfer the mixture to a MGTM SV column. Centrifuge for 1 min. Discard the pass-through and re-insert the MGTM SV column into the Collection Tube.
- Add 700 ul of Buffer NW to the MGTM SV column. Centrifuge for 30 sec. Discard the pass-through. Reinsert the MGTM SV column into the Collection Tube.
- Centrifuge for additional 1 min to remove residual wash buffer. Transfer the MGTM SV column to a new 1.5 ml tube.
- Apply 30ul of Buffer EB to the center of the membrane in the MGTM SV column, let stand for 1 min, and centrifuge for 1 min.
6. PCR purification
Materials
- AccuPrep® PCR Purification Kit - BIONEER
Procedure
- Add 5 volumes of PB Buffer to 1 volume of the PCR reaction.
- Apply the sample to the Binding column tube to bind DNA.
- Centrifuge for 30-60 sec to make the sample pass through the Binding column tube.
- Discard flow-through and place the Binding column tube in the same tube.
- Add 500μl of WB Buffer to the Binding column tube and centrifuge for 30-60 sec to wash.
- Discard flow-through and place the Binding column tube in the same tube again.
- Centrifuge the Binding column tube for an additional 1min for drying.
- Place the Binding column tube in a clean 1.5 ml tube.
- Add 30μl of EL Buffer to the center of the Binding column filter, and let the column stand for 1 min.
- Centrifuge for 1 min to elute.
7. Mini-prep (Plasmid extraction)
Materials
- AccuPrep® plasmid mini extraction Kit – BIONEER
- Buffer 1 - Resuspension buffer
- Buffer 2 - Lysis buffer
- Buffer 3 - Neutralization buffer
- Buffer 4 - Washing buffer
- Buffer 5 - Elution buffer
Procedure
- Add 250ul of Buffer 1 to the collected cells and completely resuspend by vortexing or pipetting.
- Add 250ul of Buffer 2 and mix by inverting the tube 3-4 times gently.
- Add 350ul of Buffer 3 and immediately mix by inverting the tube 3-4 times gently.
- Centrifugation the tube at 13000rpm, 4℃ for 10min.
- Transfer the cleared lysate to the DNA binding column tube and centrifuge 1min pour off the flow-through and re-assemble the DNA binding filter column with the 2mL collection tube.
- Add 700ul of Buffer 4 to the DNA binding column tube and centrifuge 1min. Pour off the flow-through and re-assemble the DNA binding filter column with the 2mL collection tube.
- Dry by additional centrifuge 1min.
- Transfer the DNA binding filter column to the new 1.5mL EP tube.
- Add 30ul of buffer 5 to the DNA binding filter column and wait 1min.
- Elute the plasmid DNA by centrifuge 1min.
8. Overlapping Extension PCR
Materials
Procedure
9. Preparation of cells for protein expression check
Materials
Procedure
1) Cell pre-culture
- Seed 10ul of cells to 3mL of LB (1% of appropriate antibiotics)
- Culture at 37℃ for 16hr
2) Induction
- Seed 500ul of cells to 3mL of LB (1% of appropriate antibiotics)
- Culture at 30℃ and 37℃ for 2hr.
- When the O.D. value is between 0.4 and 0.7, put the proper inducer with the volume set for each concentration.
3) Sampling
- 1. After proper induction time, check O.D. value
- 2. Gather 1010 of cells and centrifuge cells at 4℃ for 15 min.
- 3. Remove supernatant and resuspend cells with 1ml lysis buffer.
- 4. Transfer the sample to the new 1.5ml ep-tube and add 1ul lysozyme.
- 5. Incubate on 37℃ rotor for an hour.
- 6. After incubation, sonicate the cell. (Pulse on 20sec, off 40sec for 5 times, 13% amplitude)
- 7. Centrifuge 13,000rpm for 1min
- 8. Separate supernatant (soluble fraction) and pellet (insoluble fraction)
10. SDS PAGE
We did sodium dodecyl sulfate polyacrylamide gel electrophoresis according to cold spring harbor protocol. ▶▶Click here to show 'cold spring harbor protocol'
Protocol 11 title