Team:NTU Taiwan/index.html
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- | <h1 class=" rainbow-text header"> | + | <h1 class=" rainbow-text header">iGEM-NTU-Taiwan YeasTherm</h1> |
<p class="header container"> | <p class="header container"> | ||
<img class="spin" alt-src="images/LaboratoryLevels.png" src="/wiki/images/9/91/NTU_TAIWAN_LaboratoryLevels.png"><br/> | <img class="spin" alt-src="images/LaboratoryLevels.png" src="/wiki/images/9/91/NTU_TAIWAN_LaboratoryLevels.png"><br/> | ||
National Taiwan University<br/> | National Taiwan University<br/> | ||
- | Working | + | Working on Thermogenic Yeast<br/> |
- | Apps with | + | Apps with concept of iGEM competition and synthetic biology. |
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<h1 class="header">Applications</h1> | <h1 class="header">Applications</h1> | ||
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- | + | <p class="header" style="margin: 0"> Being an special lipid productive yeast, <i>Rhodotorula glutinis</i> has strong potentiality to become an extraordinary bio-heating device. Let's find out! </p> | |
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- | <br/><p><b>PCR</b></p | + | <br/><p><b>PCR</b></p> |
- | + | 1: Design of appropriate forward and reverse primers<br/> | |
- | + | 2: Prepare our template<br/> | |
- | + | 3: Prepare the PCR mix. (Kapa Hifi PCR kit.)<br/> | |
- | + | 4: Run PCR<br/> | |
- | + | 5: Examine the results by electrophoresis<br/> | |
- | Note: If the template is genomic DNA, we would adjust the annealing temperature at 45°C. It is because the copy number of target gene may be low. We use this annealing temp when perform PCR of Tir1, 26s, 5.8s ITS | + | Note: If the template is genomic DNA, we would adjust the annealing temperature at 45°C. It is because the copy number of target gene may be low. We use this annealing temp when perform PCR of Tir1, 26s, 5.8s ITS<br/><br/> |
- | <br/><p><b>Construction of our parts</b></p>< | + | <br/><p><b>Construction of our parts</b></p><p> |
- | + | 1: We design primers for parts with prefix and suffix.<br/> | |
- | + | 2: Perform PCR and cleanup the PCR product<br/> | |
- | + | 3: Before insert our parts into standard backbone, pSB1C3, we perform RE digestion to make sticky ends of both inserts and backbones.<br/> | |
- | + | 4: Ligation of inserts and backbones<br/> | |
- | + | 5: Transform our ligation products into DH5α and streak the transformed DH5α on LB agar plate with chloramphenicol.<br/> | |
- | + | 6: Inoculate single colony into broth with chloramphenicol.<br/> | |
- | + | 7: Miniprep the plasmid DNA from the overnight broth culture.<br/> | |
- | + | 8: Confirm the products by both RE digestion and PCR sequencing<br/></p> | |
<p><b>Point mutation protocol</b></p> | <p><b>Point mutation protocol</b></p> |
Latest revision as of 04:22, 28 September 2013