"
Team:DTU-Denmark/Methods/Notebook
From 2014.igem.org
Tbjohannesen (Talk | contribs) |
Tbjohannesen (Talk | contribs) |
||
| Line 292: | Line 292: | ||
<ul><li><b>13th of June</b>: | <ul><li><b>13th of June</b>: | ||
</li></ul> | </li></ul> | ||
| - | <p>< | + | <p> |
| - | Participants: Casper and Kristian K | + | <b>Participants:</b> Casper and Kristian K<br> |
| - | Purpose: Preparing linearized backbone (pSB1K3) from iGEM biobrick part for USER cloning by means of PCR | + | <b>Purpose:</b> Preparing linearized backbone (pSB1K3) from iGEM biobrick part for USER cloning by means of PCR<br> |
| - | Results: Amplification was unsuccessful - no band were detected when running the PCR samples on a 1% agarose gel | + | <b>Results:</b> Amplification was unsuccessful - no band were detected when running the PCR samples on a 1% agarose gel<br> |
A PCR were made to amplify and attach tails for USER cloning to the linearized backbone (pSB1K3) using the primers P1 and P2. Two reactions were prepared according to the table below | A PCR were made to amplify and attach tails for USER cloning to the linearized backbone (pSB1K3) using the primers P1 and P2. Two reactions were prepared according to the table below | ||
| - | |||
</p> | </p> | ||
</div> | </div> | ||
| Line 306: | Line 305: | ||
</li></ul> | </li></ul> | ||
<p> | <p> | ||
| - | Participants: | + | <b>Participants:</b> <br> |
| - | Purpose: Investigating the success of the PCR the day before by gel electrophoresis | + | <b>Purpose:</b> Investigating the success of the PCR the day before by gel electrophoresis<br> |
| - | Results: PCR amplification were unsuccessful - no bands were detected | + | <b>Results:</b> PCR amplification were unsuccessful - no bands were detected<br> |
PCR products from 130614 was run on a 1% agarose + 1X TAE buffer GEL. | PCR products from 130614 was run on a 1% agarose + 1X TAE buffer GEL. | ||
Revision as of 12:45, 15 August 2014
- Home
- Overview
- Methods
- Achievements
- Team
At the Giant Jamboree, we received a gold medal and an Interlab Study Award. We also won the Overgrad Best Parts Collection.
Notebook
[edit] Chronological notebook
- 13th of June:
Participants: Casper and Kristian K
Purpose: Preparing linearized backbone (pSB1K3) from iGEM biobrick part for USER cloning by means of PCR
Results: Amplification was unsuccessful - no band were detected when running the PCR samples on a 1% agarose gel
A PCR were made to amplify and attach tails for USER cloning to the linearized backbone (pSB1K3) using the primers P1 and P2. Two reactions were prepared according to the table below
- 14th of June:
Participants:
Purpose: Investigating the success of the PCR the day before by gel electrophoresis
Results: PCR amplification were unsuccessful - no bands were detected
PCR products from 130614 was run on a 1% agarose + 1X TAE buffer GEL.
5ul PCR product + 1ul loading dye was loaded on the gel as well as 4ul ladder 1 kb.
- 27th of June:
Fluorescence We did blabla, no fluorescence.
- 1st of July:
Headline EtOH resistance assay was continued in a narrow concentration range (Jan).
E. coli (DH5alpha) cells were transformed using BioBricks required for EtOH production (Aleksandra).
O/N cultures of E. coli and B. subtilis were set up to continue with the experiments tomorrow (Harry).
