"
Team:Yale/Our Project/Notebook/Week 4
From 2010.igem.org
(Difference between revisions)
| Line 75: | Line 75: | ||
<td>Primers</td> <td>phsC_F & phsC_R</td> <td>phsABC_F & phsAB_R</td> <td> phsABC_F & phsC_R</td> | <td>Primers</td> <td>phsC_F & phsC_R</td> <td>phsABC_F & phsAB_R</td> <td> phsABC_F & phsC_R</td> | ||
</tr> | </tr> | ||
| + | </table> | ||
<li> Chilled tubes on ice, then added 0.5 uL of Phusion DNA polymerase and put in thermocycler. </li> | <li> Chilled tubes on ice, then added 0.5 uL of Phusion DNA polymerase and put in thermocycler. </li> | ||
<li> Prior to designing thermocycler protocol, used oligocalc to get the following Tm values for the primers. </li> | <li> Prior to designing thermocycler protocol, used oligocalc to get the following Tm values for the primers. </li> | ||
| Line 94: | Line 95: | ||
6. Hold--indefinitely at 4˚C<br/> | 6. Hold--indefinitely at 4˚C<br/> | ||
<b> Gel of PCR Products </b> <br/> | <b> Gel of PCR Products </b> <br/> | ||
| - | + | Ran PCR products on an 0.8% agarose gel with 10 uL of ethidium bromide. Loaded 1 uL of each sample with 9 uL of water and 2 uL of loading buffer. Ran gel until done at 60 V, but had difficulty imaging so left aside to deal visualize the next day, unaware that it would spread. <br/> | |
| + | </ul> | ||
<!------------- Monday -------------> | <!------------- Monday -------------> | ||
Revision as of 09:46, 27 October 2010
our project
lab notebook: week 4 (6/28 -7/4)
- Monday 6/28--PCR amplification of thiosulfate reductase operon phsABC See more/less
- Tuesday short content See more/less
- Wednesday short content See more/less
- Thursday short content See more/less
- Fridays short content See more/less
- Saturday short content See more/less
- Sunday short content See more/less
