Revision as of 03:49, 19 September 2012

Results and Characterisation

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Heme Oxygenase

We produced a Heme oxygenase that was codon optimize for E. coli. The Gibson assembly of the T7 promoter containing Heme Oxygenase was successful. The transformation was successful with numerous colonies grown using Chloramphenicol as the selecting agent. Six colonies were selected and then they were sequenced and digested with EcoR1 and Spe1. The sequencing suggested that all of the colonies contained the plasmid with a Heme oxygenase identical to the original protein sequence. The gel containing the digested Heme Oxygenase bearing plasmid can be seen in Figure 1.

Figure 1: The restriction digest showing the linearised plasmid backbone (Black Box) and the heme oxygenese gene (Green Box)

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 <p>We produced a Heme oxygenase that was codon optimize for <i>E. coli</i>. The Gibson assembly of the T7 promoter containing Heme Oxygenase was successful. The transformation was successful with numerous colonies grown using Chloramphenicol as the selecting agent. Six colonies were selected and then they were sequenced and digested with EcoR1 and Spe1. The sequencing suggested that all of the colonies contained the plasmid with a Heme oxygenase identical to the original protein sequence. The gel containing the digested Heme Oxygenase bearing plasmid can be seen in Figure 1.</p>
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Team:Macquarie Australia/Results

From 2012.igem.org

Revision as of 03:49, 19 September 2012

Results and Characterisation

Heme Oxygenase

Bacteriophytochrome

Heme Oxygenase

Bacteriophytochromes