Difference between revisions of "Team:MIT/pdestmcherry"
| Line 17: | Line 17: | ||
<li>5x LR Clonase II</li> | <li>5x LR Clonase II</li> | ||
<li>Proteinase K </li> | <li>Proteinase K </li> | ||
| + | </p> | ||
<p> <h5>Procedure</h5> | <p> <h5>Procedure</h5> | ||
| − | + | Into each tube: </li> SUBLISTS????????? | |
<li>1 µl of the promoter pENTR </li> | <li>1 µl of the promoter pENTR </li> | ||
<li>1 µl of the gene pENTR </li> | <li>1 µl of the gene pENTR </li> | ||
<li>1 µl of the pDEST-mCherry </li> | <li>1 µl of the pDEST-mCherry </li> | ||
| − | + | Add 1 µl of TE </li> | |
| − | + | Add 1 µl of LR clonase (kept in -80)</li> | |
| − | + | Cap tubes, flick to mix and pulse-spin to collect liquid at the bottom</li> | |
| − | + | Incubate between 12-24 hours at room temperature. </li> | |
| + | </p> | ||
Revision as of 05:56, 8 October 2016
I NEEDED A PAGE!!!!!!!
During the insertion of the the pENTR constructs into the pDEST, the mCherry gets cut out of the plasmid. When transformed into eColi on plates containing Ampicillin, the mCherry acts as a negative screening tool for choosing colonies that contain the properly-assembled plasmid of choice. the pDEST plasmid here is designed with the express purpose of distribution for use by other teams and scientists.
.Using the pDEST with mCherry is extremely similar to normal ligation reaction, transformations, and plating protocols.
<looool
Many thanks are owed to the Tufts iGEM 2016 team, for agreeing to test our construct for us!
Materials
Procedure
Into each tube: </li> SUBLISTS?????????
Add 1 µl of TE </li> Add 1 µl of LR clonase (kept in -80)</li> Cap tubes, flick to mix and pulse-spin to collect liquid at the bottom</li> Incubate between 12-24 hours at room temperature. </li>
