Team:UT Dallas/week5
From 2011.igem.org
Line 2: | Line 2: | ||
<table> | <table> | ||
- | <tr><td valign='top'> | + | <tr><td valign='top'>1/8/11</td><td valign='top'> |
- | + | Miniprep<br> | |
- | + | Observations: i2.11.6 grew, i2.10.7 no growth<br> | |
- | + | Making glycerol stock<br> | |
- | + | Dissolving and diluting primers (10 pmol/ µL)<br> | |
- | + | PCR and gel electrophoresis and purification<br> | |
- | + | At this stage we have both the FOFr and CheZ* with XbaI and SteI restriction sites.<br>Our next goal will be to insert each part into a vector backbone so they will be ready<br>for addition of the ToxR and Ctx genes. Once these two fusion products are made,<br>we hope to transform and test whether local motion can be inhibited with CheZ and the<br>receptor combo | |
</td></tr><tr><td valign='top'> </td><td valign='top'> </td></tr><tr><td valign='top'> | </td></tr><tr><td valign='top'> </td><td valign='top'> </td></tr><tr><td valign='top'> | ||
- | + | 2/8/11 | |
</td><td valign='top'> | </td><td valign='top'> | ||
- | + | Gel electrophoresis and purification<br> | |
+ | Dephosphorylation for 1 hour at 37 degrees Celsius, PCR purify<br> | ||
+ | Ligation at 16 degrees Celsius overnight<br> | ||
+ | We added both CheZ* and FGFR each into its own vector and if the ligation just performed works we will have 2 new biobricks.<br>The phosphorylation was done to prevent ligase from reannealing the X and S site on the vector.<br>This means only the phosphate on the insert can be used to connect the 2 DNA sequences. | ||
</td></tr><tr><td valign='top'> </td><td valign='top'> </td></tr><tr><td valign='top'> | </td></tr><tr><td valign='top'> </td><td valign='top'> </td></tr><tr><td valign='top'> | ||
- | + | 3/8/11 | |
</td><td valign='top'> | </td><td valign='top'> | ||
- | + | Transformation of FOFR and CheZ*, DH5a, 50 µL 2 µL DNA at 37 degrees Celsius | |
</td></tr><tr><td valign='top'> </td><td valign='top'> </td></tr><tr><td valign='top'> | </td></tr><tr><td valign='top'> </td><td valign='top'> </td></tr><tr><td valign='top'> | ||
- | + | 4/8/11 | |
</td><td valign='top'> | </td><td valign='top'> | ||
- | + | Incubation in 3 mL and chlora at 37 degrees Celsius and 220 rpm<br> | |
- | + | Plating CheZ (K283006) and ToxR (J07009)<br> | |
+ | Dephosphorylation for 1 hour at 37 degrees Celsius, PCR purify | ||
</td></tr><tr><td valign='top'> </td><td valign='top'> </td></tr><tr><td valign='top'> | </td></tr><tr><td valign='top'> </td><td valign='top'> </td></tr><tr><td valign='top'> | ||
- | + | 5/8/11 | |
</td><td valign='top'> | </td><td valign='top'> | ||
- | + | Making glycerol stock<br> | |
+ | Miniprep<br> | ||
+ | Incubation in 3 mL LB carb at 37 degrees Celsius and 220 rpm overnight<br> | ||
+ | Test digestion ( 1 hour and 30 minutes)- about 200 ng of DNA<br> | ||
+ | Gel electrophoresis<br> | ||
+ | Observations: i2.15.16 looks positive, the rest are negative | ||
</td></tr><tr><td valign='top'> </td><td valign='top'> </td></tr><tr><td valign='top'> | </td></tr><tr><td valign='top'> </td><td valign='top'> </td></tr><tr><td valign='top'> | ||
- | + | 6/8/11 | |
</td><td valign='top'> | </td><td valign='top'> | ||
- | + | Glycerol stock and miniprep</td></tr> | |
</table> | </table> |
Latest revision as of 00:55, 28 September 2011
Week 5
1/8/11 |
Miniprep |
2/8/11 |
Gel electrophoresis and purification |
3/8/11 |
Transformation of FOFR and CheZ*, DH5a, 50 µL 2 µL DNA at 37 degrees Celsius |
4/8/11 |
Incubation in 3 mL and chlora at 37 degrees Celsius and 220 rpm |
5/8/11 |
Making glycerol stock |
6/8/11 | Glycerol stock and miniprep |