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

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                                     <h5 class="question">How to prove our design?</h5>
 
                                     <h5 class="question">How to prove our design?</h5>
 
                                     <p class="pcontent">We designed a total solution test to verify the function of our whole construction.  
 
                                     <p class="pcontent">We designed a total solution test to verify the function of our whole construction.  
                                         We incubate the constructed strains in adjacent M9 medium that contains 0.4% xylose as its sole carbon source.  
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                                         We incubate the constructed strains in modified M9 medium that contains 0.4% xylose as its sole carbon source.  
 
                                         The construction is designed to consume xylose as energy source and as a material for Calvin-Bensson cycle.  
 
                                         The construction is designed to consume xylose as energy source and as a material for Calvin-Bensson cycle.  
 
                                         We then measure the optical intensity (O.D. 600) to characterize the cell growth. At a fixed time interval,  
 
                                         We then measure the optical intensity (O.D. 600) to characterize the cell growth. At a fixed time interval,  
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                                     <h5 class="question">How we determine its function?</h5>
 
                                     <h5 class="question">How we determine its function?</h5>
 
                                     <p class="pcontent">We measure the fluorescence intensity of the plasmid in different pH environment to  
 
                                     <p class="pcontent">We measure the fluorescence intensity of the plasmid in different pH environment to  
                                         determine its promoter activity. We incubate the bacteria in pH adjacent M9 medium and  
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                                         determine its promoter activity. We incubate the bacteria in pH modified M9 medium and  
 
                                         measure the fluorescence intensity (absorbance: 480 nm, excitation: 510 nm) in a short period of time.
 
                                         measure the fluorescence intensity (absorbance: 480 nm, excitation: 510 nm) in a short period of time.
 
                                     </p>
 
                                     </p>

Revision as of 02:34, 14 October 2018

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igem.ncku.tainan@gmail.com
No.1, Daxue Rd., East Dist., Tainan City 701, Taiwan (R.O.C.)