Team:BostonU/Methodology

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BostonU iGEM Team: Welcome


Methodology



Making Destination Vectors and MoClo Parts

    Building Destination Vectors

      In order to generate MoClo Destination Vectors (DV)s, we had to add the alpha fragment of lacZ to BioBrick backbones where DNA parts are normally inserted. First, we PCR amplified the alpha lacZ fragment with primers designed to add both the MoClo fusion sites and type IIs restriction sites to it.

      The amplified products and the backbones were digested with SpeI and ligated together to generate the Destination Vectors (DV)s. We performed blue-white screening to select the correct DVs and selected the blue colonies for mini preps. These were sent for sequencing to verify the correct orientation of the MoClo sites and type IIS restriction sites.



      Level 0 DVs contain Chloramphenicol resistance on the backbone (BioBrick backbone used: pSB1C3) and a BsaI site followed by a Bpil site. Level 1 DVs contain Kanamycin resistance on the backbone (BioBrick backbone used: pSB1K3) and a Bpil site followed by a BsaI site. Level 2 DVs contain Ampicillin resistance on the backbone (BioBrick backbone used: pSB1A3) and a BsaI site followed by a Bpil site.