Difference between revisions of "Team:UCLA/Notebook/Honeybee Silk/13 July 2015"
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| + | ='''Visualization'''= | ||
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| + | I ran each of the sample on a 1% agarose gel against a 1kB ladder for 20 minutes. | ||
| + | Expected band sizes: ~1000bp | ||
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| + | [[File:Gel_7-13.tif|200px|thumb|left|alt text]] | ||
=Testing competency of BL21 cells from 7/12= | =Testing competency of BL21 cells from 7/12= | ||
Revision as of 17:45, 14 July 2015
Contents
Colony PCR of 7/12 Transformation
- The transformation was successful for the 3:1 ligated products plates. I picked 3 colonies off the plate and suspended each in 100uL of ddH2O.
- Using APEX Taq Red Mastermix
| Component | Volume (out of 25uL) |
|---|---|
| APEX Taq Red Mastermix | 12.5uL |
| 10mM primer 10 | 1.25uL |
| 10mM primer 11 | 1.25uL |
| Transformed Cells | 1uL |
| Nuclease Free Water | 9uL |
Program
| Step | Temperature | Time |
|---|---|---|
| Initial Denaturation | 95C | 30s |
| Cycles(x30) | 95C | 10s |
| Annealing | 67C | 20s |
| Extension | 70C | 30s |
| Final Extension | 70C | 2 min |
| Hold | 14C | Hold |
Visualization
I ran each of the sample on a 1% agarose gel against a 1kB ladder for 20 minutes. Expected band sizes: ~1000bp
Testing competency of BL21 cells from 7/12
- Used puc 19 vector at 50 picograms/ul to test transformation efficiency.
- Added 2 ul of puc 19 to 50 ul of competent BL21 cells
- Used this NEB protocol to transform with our BL21 cells.
- Plated 10% of the cells on a warm amp plate and put plate in at 4 pm 7/13