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

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                                         We initially decided to test its function by HPLC to measure the amount of RuBP
 
                                         We initially decided to test its function by HPLC to measure the amount of RuBP
 
                                         inside the cell. Our instructors pointed out some difficulties in HPLC
 
                                         inside the cell. Our instructors pointed out some difficulties in HPLC
                                         measurement such as excessive noise signal in our sample.We, therefore,
+
                                         measurement such as excessive noise signal in our sample. We, therefore,
 
                                         determined to test its function with a toxicity test. The product of PRK-RuBP
 
                                         determined to test its function with a toxicity test. The product of PRK-RuBP
 
                                         cannot be metabolite by wild-type <i>E. coli</i>. The accumulation of RuBP
 
                                         cannot be metabolite by wild-type <i>E. coli</i>. The accumulation of RuBP
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                                         shows a
 
                                         shows a
 
                                         little growth arrest comparing to the strain without plasmid. The growth of it
 
                                         little growth arrest comparing to the strain without plasmid. The growth of it
                                         exceed that of PRK expressed in pSB1C3. We can regulate the expression of PRK
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                                         exceeds that of PRK expressed in pSB1C3. We can regulate the expression of PRK
 
                                         via
 
                                         via
 
                                         high or low copy number plasmid to optimize the growth and carbon fixation
 
                                         high or low copy number plasmid to optimize the growth and carbon fixation
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                                     <p class="pcontent">
 
                                     <p class="pcontent">
                                         The test samples below were incubated in an altered M9 medium which substitute
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                                         The test samples below were incubated in an altered M9 medium which substitutes
 
                                         glucose to xylose. 1/1000 of LB medium was added to support some rare elements.
 
                                         glucose to xylose. 1/1000 of LB medium was added to support some rare elements.
 
                                         Since the concentration of LB medium is too low, it doesn’t contribute the
 
                                         Since the concentration of LB medium is too low, it doesn’t contribute the
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                                         source
 
                                         source
 
                                         provided in our medium) as its carbon source. Although some native <i>E. coli</i>
 
                                         provided in our medium) as its carbon source. Although some native <i>E. coli</i>
                                        pathway
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                                        pathway
 
                                         may utilize CO<sub>2</sub> (such as lipid synthesis), the amount is too small
 
                                         may utilize CO<sub>2</sub> (such as lipid synthesis), the amount is too small
 
                                         to consider.
 
                                         to consider.

Revision as of 12:32, 16 October 2018

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