Team:Harvard/Template:NotebookDataJuly

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July 9

Team ZF

Isothermal Assembly

We performed an isothermal assembly in order to insert omega+zif268 into the plasmid containing the spec backbone.

  • The concentration of the plasmid (previously prepared) was 157.4 ng/ul.
  • The concentration of the w+zif268 was 54.3 ng/ul.

Using our protocols we determined we needed:

  • 0.63 ul backbone (length: ~2.2 kb)
  • 0.59 ul w+zif268 (length: ~0.7 kb)
  • 2.78 ul water
  • 15.0 ul isothermal assembly solution

Transformation of electro-competent E. coli

We electroporated our cells so they would take up the plasmids, using:

  • 1.0 ul DNA
  • 40.0 ul cells
  • 500 ul LB

We plated the cells, using this protocol, on spec plates, one of which contained 50 ul of cells and the other 150 ul of cells. The cells have been incubated at 37*, and will be left there overnight. Cells that have taken up the plasmid have spec-resistance and should be able to survive. Tomorrow, we will be picking colonies and performing PCR on them to determine whether they contain w+zif268.

Team Wolfe

  • MAGE3 plates look good--we'll choose colonies for sequencing on Monday.
  • Transformation of selection strain with Vatsan's plasmid:
    • We're curious to see whether Vatsan's plasmid (Zif268 omega, ZFB, wp, hisura) will have an effect on the (∆HisB)∆pyrF∆rpoZ strain's growth despite the seemingly intact HisB.
    • Transformed mid-log selection strain (reinoculated from overnight culture) with about 100ng of Vatsan's plasmid following standard procedure.
    • After 2 hr recovery plated on amp plates with 100µL or 1mL