Team:TzuChiU Formosa/Project
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+ | <font size="4"><b>Group one: pSB1C3</b></font> | ||
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+ | We have successfully obtained the pSB1C3 vector and the insert we have designed (BBa_K1222887、BBa_K1222886、BBa_K1222885、BBa_K1222884、BBa_K1222883、BBa_K1222882、 BBa_K1222881). After ligation, we transformed the plamid think DH5α. | ||
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+ | <img src="https://static.igem.org/mediawiki/2013/4/44/Result_1.png" height="500px"> | ||
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+ | <img src="https://static.igem.org/mediawiki/2013/3/38/Result_2.png" width="400px"> | ||
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+ | <li>We have Picked a single colony of the bacteria cultured and performed streaking. According to each quadrant of single colony, we have done a colony PCR but only a primer dimer band was shown. We conjecture that this is because the specificity of the primer is not high enough. | ||
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+ | <img src="https://static.igem.org/mediawiki/2013/7/75/Result_3.png" width="700px"> | ||
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+ | While performing the experiment above, we have also attempted to clone lac I. Firstly, we designed a primer with regard to lac I on the pET11d and used TGradient Thermocycler to test several annealing temperatures (Tm) but unfortunately, we did not succeed. We assume that this is because the sequence for lac I is too large hence, it cannot be cloned out at once. We then tried overlapping PCR and designed several groups of primers. Again, we did not manage to succeed. | ||
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+ | <font size="4"><b>Group two: pET11d</b></font> | ||
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+ | Since the pET11d plasmid contains the lac I gene, so to make up for the previous group (group 1), we have decided to use pET11d. Successfully we managed to get the pET11d vector and our designed antisense insert (BBa_K1222994, BBa_K1222995, BBa_K1222996, BBa_K1222997, BBa_K1222998, BBa_K1222988, BBa_K1222989), which includes GFP and Ampicillin. After ligation, we transformed it into BL21 but nothing grew on the agar plate. The control group (Ampicillin free) proved that there is nothing wrong with the competent cell and in fact we have obtained a complete plasmid from digestion. Therefore, we assume the reasons could be the following: | ||
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+ | a. Unsuccessful ligation | ||
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+ | b. The size of the plasmid is too large | ||
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+ | c. Probably BL21 already contains a plasmid (T7 polymerase sequence) therefor the chances of it would not accept another plasmid | ||
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Revision as of 23:28, 27 September 2013