Difference between revisions of "Team:NCKU Tainan/Design"

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                                         The sequence and the size of RbcL is much larger than other subunit,  
 
                                         The sequence and the size of RbcL is much larger than other subunit,  
 
                                         so we separated rbcL from rbcX and rbcS subunits. RbcX and rbcS is separated by a rbs (B0034) for the convenience of construction.  
 
                                         so we separated rbcL from rbcX and rbcS subunits. RbcX and rbcS is separated by a rbs (B0034) for the convenience of construction.  
                                         We attached two different promoters upstream of the rubisco. They are PLacI and PT7 promoter.  
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                                         We attached two different promoters upstream of the rubisco. They are PLacI and P<sub>T7</sub> promoter.  
 
                                         Since we would like to increase the expression of this protein in the metabolic pathway,  
 
                                         Since we would like to increase the expression of this protein in the metabolic pathway,  
 
                                         we would like to test various promoter combination to find out most efficient combination for our pathway.
 
                                         we would like to test various promoter combination to find out most efficient combination for our pathway.
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                                     <p class="pcontent">We first extracted whole genome DNA from <i>E. coli</i> MG1655 and amplify both promoters by PCR  
 
                                     <p class="pcontent">We first extracted whole genome DNA from <i>E. coli</i> MG1655 and amplify both promoters by PCR  
 
                                         using primers that contains HindIII and SpeI.  
 
                                         using primers that contains HindIII and SpeI.  
                                         We then exchanged the promoter with the previously constructed plasmid that contains PT7 and sfGFP.  
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                                         We then exchanged the promoter with the previously constructed plasmid that contains P<sub>T7</sub> and sfGFP.  
 
                                         We initially transformed the constructed plasmid into DH5 alpha for colony screening.  
 
                                         We initially transformed the constructed plasmid into DH5 alpha for colony screening.  
 
                                         We then transformed the plasmid into BL21(DE3) to test its function.
 
                                         We then transformed the plasmid into BL21(DE3) to test its function.

Revision as of 14:15, 29 September 2018

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