Team:UC Davis/notebook/assembly.html

From 2010.igem.org

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**Click on the individual pieces above to view how we ligated them together.** <p><br />
**Click on the individual pieces above to view how we ligated them together.** <p><br />
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<a name="plasmid"></a><p class="header"><b>Placing them into individual plasmids</b></a><p>
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<a name="plasmid"></a><p class="header"><b>Next Mission: Placing them into only two plasmids</b></a><p>
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<li>After we have created the individual pieces, we must ligate the composite parts together into a total of two plasmids. </li>
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<img src="https://static.igem.org/mediawiki/2010/3/36/Plasmid1.jpg"><br />
<img src="https://static.igem.org/mediawiki/2010/3/36/Plasmid1.jpg"><br />

Revision as of 21:02, 27 October 2010

Assembly Workplans

Miscellaneous Parts


Genetic Circuit


**Click on the individual pieces above to view how we ligated them together.**


Next Mission: Placing them into only two plasmids



Sample Ligation Procedure

Because the initiator is one of the smaller constructs, we have decided to use this as an example to illustrate the utmost basic workplan in greater detail.

Starting Up

  • Hydrated parts: BBa_B0034, BBa_C0051, BBa_B0015, BBa_R0082.
  • Transformed these parts into DH5α competent cells.


RBS to BBa_C0051


  • Ligate the RBS and BBa_C0051 fragments together and transform on carb plates.
  • Depending on the outcome of visible colonies on the experimental and control plates, a PCR screening may be needed.


Assembly notes
  • It is most practical to cut RBS as a vector because RBS is less than 100 bp long as an insert, making it hard to see and extract on the gel.
  • The sticky ends from the XbaI and SpeI, when ligated together, will form an 8 bp scar. Thus, XbaI and SpeI will no longer be able to cut here.

'RBS & BBa_C0051' to Terminator
  • Cultured cells that have parts: 'RBS & BBa_C0051', BBa_B0015
  • Miniprepped 'RBS & BBa_C0051' and BBa_B0015


  • Ligate the fragments together and transform on kan plates.
  • Depending on the outcome of visible colonies on the experimental and control plates, a PCR screening may be needed.


Assembly notes

  • It is most practical to cut BBa_B0015 as the vector because it is only 130 bp long. It would be hard to see on a gel.

'RBS & BBa_C0051 & stop' to BBa_R0082
  • Cultured cells that have parts: 'RBS & BBa_C0051 & stop', BBa_R0082
  • Miniprepped 'RBS & BBa_C0051& stop' and BBa_R0082


  • Ligate the fragments together and transform on carb plates.
  • Depending on the outcome of visible colonies on the experimental and control plates, a PCR screening may be needed.


Assembly notes
  • The promoter had to be cut as a vector because it is only 108 bp by itself.
We would like to take a moment to thank all of our sponsors for their very generous donations, as we could not have done this without your help!

We would also like to thank and acknowledge:
Our Advisors
Marc Facciotti
Ilias Tagkopoulos
Technical Guidance
David Larsen
Andrew Yao
Visiting iGEMer
Jia Li of Zhejiang University (TEAM ZJU-China)
cI Promoter Screen
Drew Endy - Stanford
Thomas Schneider - NIH
Want to sponsor us? Send an email to mtfacciotti@ucdavis.edu to discuss various ways you can help! :)

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