Team:Korea U Seoul/Project/Design Parts
From 2012.igem.org
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<b> A. Ax21 Producing Bacteria </b> | <b> A. Ax21 Producing Bacteria </b> | ||
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<br>Figure.1: Plasmid construction of pAT – Ax21 | <br>Figure.1: Plasmid construction of pAT – Ax21 | ||
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<b> B. Ax21 Detecting Bacteria </b> | <b> B. Ax21 Detecting Bacteria </b> | ||
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<br>Figure2: Plasmid construction of Rice Guardian | <br>Figure2: Plasmid construction of Rice Guardian | ||
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Revision as of 14:26, 26 September 2012
Rice Guardian
Our team aims to make 3 engineered bacteria in Rice Guardian project. In order to detect Ax21, we need to produce it. First, we created Ax21 producing bacteria. Second, we have to create an engineered E. coli which detects Ax21. Lastly we created an engineered E. coli which kills Xanthomonas oryzae KACC10331 in addition to detecting it, an improved bacterium. (still working on)
Strian used for Rice Guardian was Xanthomonas oryzae KACC10331, a specie of Xanthomonas oryzae pv oryzae populating in Korea. A Korean researcher named Ax21 detecing gene Col R and Col S, a different nomination of Rax R and Rax H which is commonly used. We used Xanthomonas oryzae KACC10331 and Col R, S instread of Xanthomonas oryzae pv oryzae and Rax R, H in our project. Even though Col R and Col S was used, Rax R and Rax H will be used interchangeably since they are more commonly used.
A. Ax21 Producing Bacteria
Figure.1: Plasmid construction of pAT – Ax21
Ax 21 is required for our engineered bacteria to detect Xanthomonas oryzae KACC10331. So we produced Ax21 producing bacteria. pAT is a promoter which is regulated by arabinose. In presence of arabinose, a promoter will operate. In absence of arabinose, a promoter will not operate. As a result of a pAT promoter, Ax21 will be displaced on the membrane surface of E. coli .
B. Ax21 Detecting Bacteria
Construction of Ax21 detecting bacteria plasmid
Figure2: Plasmid construction of Rice Guardian