Team:WashU/DesignSynecho
From 2012.igem.org
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==Rising Action== | ==Rising Action== | ||
- | + | We started to work on the gene we were going to transform E. Coli and Synechocystics early. We decided to construct 3 genes and put them in a plasmid that could homogeneously recombine in Synechocystis. The 3 genes we chose were ZCD, UGTCS2 and CrtZ. CrtZ (β-carotene hydroxylase) makes zeaxanthin from β-carotene. We wanted to include this gene even though Synechocystis produces Zeaxanthin endogenously because we wanted to make sure increase the amount of endogenously produced zeaxanthin produced so that we could produce more product. ZCD and UGTCS2 were the two enzymes that cleaved zeaxanthin to make our products. We picked a promoter that our advisers suggested because it had been shown in the Pakrasi lab to work well in Synechocystis. In between each gene we added Ribosome binding sites and restriction sites. The ribsome binding sites were necessary for the expression of our construct. The Restriction sites were added so that the genes could be easily cut out of the construct and manipulated. Our terminator was just a regular terminator we found on the parts registry. We optimized the construct for Synechocystis PCC 6803 using a program from DNA 2.0. We submitted the gene to DNA 2.0 to synthesize. | |
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==Climax== | ==Climax== |
Revision as of 17:36, 19 June 2012