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Team:Lethbridge
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<u>Red Buffer:</u> EcoRI, PstI, Control (No Enzyme)<br> | <u>Red Buffer:</u> EcoRI, PstI, Control (No Enzyme)<br> | ||
<u>Tango Buffer:</u> BcuI/SpeI, XbaI, DpnI, Control (No Enzyme><br><br> | <u>Tango Buffer:</u> BcuI/SpeI, XbaI, DpnI, Control (No Enzyme><br><br> | ||
| + | <u>Methods:</u> | ||
Set up Master Mixes: | Set up Master Mixes: | ||
<table><table border="3"> | <table><table border="3"> | ||
| Line 109: | Line 110: | ||
<tr><td>9</td><td>Empty</td></tr> | <tr><td>9</td><td>Empty</td></tr> | ||
<tr><td>10</td><td>Empty</td></tr> | <tr><td>10</td><td>Empty</td></tr> | ||
| - | </table> | + | </table><br> |
| + | Ran gel at 100V for 1 hour<br> | ||
| + | <b>Results:</b> pUC19 plasmid DNA not present at a high enough concentration to visualize by ethidium bromide staining (1kb ladder did stain). <br> | ||
| + | <b>Conclusion:</b> Will have to re-run experiment with DNA that is present at high enough concentrations to visualize by ethidium bromide staining<br> | ||
Revision as of 03:44, 14 May 2010
University of Lethbridge IGEM team
- Main
- Team
- Projects
- Notebook
- Meetings
- Parts
- Collaborations
blah balh balh
Our team is based yada yada
- Team Pics
- Tab 3
- Team bios
Team pictures
Content 3
Pics of us
Overview
- Project 1
- Porejct 2
Content 1
Content 2
Objective: Test Restriction Endonucleases for Activity
Related Information:
Endonucleases available
| Endonuclease | Optimal Buffer** | Other Buffers |
| EcoRV | None | 2xT(100%); O,G(50-100%) |
| EcoRI | Red | O(100%);R(100%)*;2xT(100%) |
| BcuI/SpeI | Tango | B(50-100%);G(50-100%) |
| XbaI | Tango | B,G,2xT(50-100%) |
| PstI | Orange | R(100%); B,G,T,2xT(50-100%) |
| DpnI | Tango | B,G(100%): O,R,2xT(50-100%) |
**Optimal Buffer from Fermentas
Use pUC19 plasmid as test, it has cut sites for EcoRI, PstI, XbaI (unsure about BcuI/SpeI, DpnI but will try anyways), and none for EcoRV
Red Buffer: EcoRI, PstI, Control (No Enzyme)
Tango Buffer: BcuI/SpeI, XbaI, DpnI, Control (No Enzyme>
Methods: Set up Master Mixes:
| Red MM | per tube (µL) | Total (µL) |
| MilliQ H20 | 13.75 | 55 |
| Red Buffer (10x) | 2 | 7 |
| pUC19 (10pg/µL) | 2 | 7 |
| Total | 19.75 | 69 |
| Tango MM | per tube (µL) | Total (µL) |
| MilliQ H20 | 13.75 | 55 |
| Tango Buffer (10x) | 2 | 7 |
| pUC19 (10pg/µL) | 2 | 7 |
| Total | 19.75 | 69 |
To each tube, add 19.75µL of master mix and 0.25µL of enzyme
Incubated reaction mixes at 37oC (Start:7:00pm; End:7:45pm)
Add 3.3µL of 6x loading dye to each reaction mixture and load 10µL final volume onto a 1% agarose (in TAE) gel.
Add 1µL of 6x loading dye to 1µL of GeneRuler 1kb ladder (at 0.5µg/µL)
Gel loading order as follows:
| Lane | Sample |
| 1 | 1kb Ladder |
| 2 | Tango Control |
| 3 | DpnI (Tango) |
| 4 | BcuI/SpeI (Tango) |
| 5 | XbaI (Tango) |
| 6 | EcoRI (Red) |
| 7 | PstI (Red) |
| 8 | Red Control |
| 9 | Empty |
| 10 | Empty |
Ran gel at 100V for 1 hour
Results: pUC19 plasmid DNA not present at a high enough concentration to visualize by ethidium bromide staining (1kb ladder did stain).
Conclusion: Will have to re-run experiment with DNA that is present at high enough concentrations to visualize by ethidium bromide staining
May 13
This is what we did today
This is where our electronic lab book data will go, gel pictures will also go here and here is an example of it:
Content 6
Content 7
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