Difference between revisions of "Team:Amoy/Notebook/Notebook"
Pheonix Wang (Talk | contribs) |
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| Line 77: | Line 77: | ||
<p class="detail_p">1. Add 20μl ddH<sub>2</sub>O to solve the dry powder.</br> | <p class="detail_p">1. Add 20μl ddH<sub>2</sub>O to solve the dry powder.</br> | ||
2. Suck 10μl of plasmid into 50μl of competent cell for transformation.</br></p> | 2. Suck 10μl of plasmid into 50μl of competent cell for transformation.</br></p> | ||
| − | <img style="width: | + | <img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/8/87/Amoy-Notebook_Node41_figure1.jpg" /> |
<p class="detail_p"></br>3. Pick a single colony from the agar plate using a sterile pipette tip. </br> | <p class="detail_p"></br>3. Pick a single colony from the agar plate using a sterile pipette tip. </br> | ||
4. Culture at 10ml LB of chloramphenicol for 12h, 37℃, 200rpm.</br> | 4. Culture at 10ml LB of chloramphenicol for 12h, 37℃, 200rpm.</br> | ||
| Line 95: | Line 95: | ||
<p class="detail_p">1. Add 20μl ddH<sub>2</sub>O to solve the dry powder</br> | <p class="detail_p">1. Add 20μl ddH<sub>2</sub>O to solve the dry powder</br> | ||
2. Suck 10μl of plasmid into 50μl of competent cell for transformation</br></p> | 2. Suck 10μl of plasmid into 50μl of competent cell for transformation</br></p> | ||
| − | <img style="width: | + | <img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/d/d9/Amoy-Notebook_node42-1.jpeg" /> |
<p class="detail_p"></br>3. Pick a single colony from the agar plate using a sterile pipette tip. </br> | <p class="detail_p"></br>3. Pick a single colony from the agar plate using a sterile pipette tip. </br> | ||
4. Culture at 10ml LB of ampicillin for 12h, 37℃, 200rpm.</br> | 4. Culture at 10ml LB of ampicillin for 12h, 37℃, 200rpm.</br> | ||
| Line 113: | Line 113: | ||
<p class="detail_p">1. Add 20μl ddH<sub>2</sub>O to solve the dry powder</br> | <p class="detail_p">1. Add 20μl ddH<sub>2</sub>O to solve the dry powder</br> | ||
2. Suck 10μl of plasmid into 50μl of competent cell for transformation</br></p> | 2. Suck 10μl of plasmid into 50μl of competent cell for transformation</br></p> | ||
| − | <img style="width: | + | <img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/e/e9/Amoy-Notebook_node43-1.jpeg" /> |
<p class="detail_p"></br>3. Pick a single colony from the agar plate using a sterile pipette tip. </br> | <p class="detail_p"></br>3. Pick a single colony from the agar plate using a sterile pipette tip. </br> | ||
4. Culture at 10ml LB of ampicillin for 12h, 37℃, 200rpm</br> | 4. Culture at 10ml LB of ampicillin for 12h, 37℃, 200rpm</br> | ||
| Line 132: | Line 132: | ||
1. Add 20μl ddH<sub>2</sub>O to solve the dry powder</br> | 1. Add 20μl ddH<sub>2</sub>O to solve the dry powder</br> | ||
2. Suck 10μl of plasmid into 50μl of competent cell for transformation</br></p> | 2. Suck 10μl of plasmid into 50μl of competent cell for transformation</br></p> | ||
| − | <img style="width: | + | <img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/c/cd/Amoy-Notebook_node44-1.jpeg" /> |
<p class="detail_p"></br> | <p class="detail_p"></br> | ||
3. Pick a single colony from the agar plate using a sterile pipette tip. </br> | 3. Pick a single colony from the agar plate using a sterile pipette tip. </br> | ||
| Line 152: | Line 152: | ||
1. Add 20μl ddH<sub>2</sub>O to solve the dry powder</br> | 1. Add 20μl ddH<sub>2</sub>O to solve the dry powder</br> | ||
2. Suck 10μl of plasmid into 50μl of competent cell for transformation</br></p> | 2. Suck 10μl of plasmid into 50μl of competent cell for transformation</br></p> | ||
| − | <img style="width: | + | <img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/e/e4/Amoy-Notebook_node45-1.jpeg" /> |
<p class="detail_p"></br> | <p class="detail_p"></br> | ||
3. Pick a single colony from the agar plate using a sterile pipette tip. </br> | 3. Pick a single colony from the agar plate using a sterile pipette tip. </br> | ||
| Line 172: | Line 172: | ||
1. Add 20μl ddH<sub>2</sub>O to solve the dry powder</br> | 1. Add 20μl ddH<sub>2</sub>O to solve the dry powder</br> | ||
2. Suck 10μl of plasmid into 50μl of competent cell for transformation</br></p> | 2. Suck 10μl of plasmid into 50μl of competent cell for transformation</br></p> | ||
| − | <img style="width: | + | <img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/4/41/Amoy-Notebook_node46-1.jpeg" /> |
<p class="detail_p"></br> | <p class="detail_p"></br> | ||
3. Pick a single colony from the agar plate using a sterile pipette tip. </br> | 3. Pick a single colony from the agar plate using a sterile pipette tip. </br> | ||
| Line 192: | Line 192: | ||
1. Add 20μl ddH<sub>2</sub>O to solve the dry powde</br> | 1. Add 20μl ddH<sub>2</sub>O to solve the dry powde</br> | ||
2. Suck 10μl of plasmid into 50μl of competent cell for transformation</br></p> | 2. Suck 10μl of plasmid into 50μl of competent cell for transformation</br></p> | ||
| − | <img style="width: | + | <img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/8/87/Amoy-Notebook_Node41_figure1.jpg" /> |
<p class="detail_p"></br> | <p class="detail_p"></br> | ||
3. Pick a single colony from the agar plate using a sterile pipette tip. </br> | 3. Pick a single colony from the agar plate using a sterile pipette tip. </br> | ||
| Line 212: | Line 212: | ||
1. Add 20μl ddH<sub>2</sub>O to solve the dry powde</br> | 1. Add 20μl ddH<sub>2</sub>O to solve the dry powde</br> | ||
2. Suck 10μl of plasmid into 50μl of competent cell for transformation</br></p> | 2. Suck 10μl of plasmid into 50μl of competent cell for transformation</br></p> | ||
| − | <img style="width: | + | <img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/1/13/Amoy-Notebook_node48-1.jpeg" /> |
<p class="detail_p"></br> | <p class="detail_p"></br> | ||
3. Pick a single colony from the agar plate using a sterile pipette tip. </br> | 3. Pick a single colony from the agar plate using a sterile pipette tip. </br> | ||
| Line 232: | Line 232: | ||
1. Add 20μl ddH<sub>2</sub>O to solve the dry powde</br> | 1. Add 20μl ddH<sub>2</sub>O to solve the dry powde</br> | ||
2. Suck 10μl of plasmid into 50μl of competent cell for transformation</br></p> | 2. Suck 10μl of plasmid into 50μl of competent cell for transformation</br></p> | ||
| − | <img style="width: | + | <img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/5/5c/Amoy-Notebook_node49-1.jpeg" /> |
<p class="detail_p"></br> | <p class="detail_p"></br> | ||
3. Pick a single colony from the agar plate using a sterile pipette tip. </br> | 3. Pick a single colony from the agar plate using a sterile pipette tip. </br> | ||
| Line 422: | Line 422: | ||
5. Link gene with terminator under 16℃ for 8 hours</br> | 5. Link gene with terminator under 16℃ for 8 hours</br> | ||
6. Transformation</br></p> | 6. Transformation</br></p> | ||
| − | <img style="width: | + | <img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/3/34/Amoy-Notebook_node35-1.jpeg" /> |
<p class="detail_p"></br> | <p class="detail_p"></br> | ||
7. Pick 8 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of chloramphenicol</br> | 7. Pick 8 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of chloramphenicol</br> | ||
| Line 446: | Line 446: | ||
5. Link gene with terminator under 16℃ for 8 hours</br> | 5. Link gene with terminator under 16℃ for 8 hours</br> | ||
6. Transformation</br></p> | 6. Transformation</br></p> | ||
| − | <img style="width: | + | <img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/8/87/Amoy-Notebook_Node41_figure1.jpg" /> |
<p class="detail_p"></br> | <p class="detail_p"></br> | ||
7. Pick 8 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of chloramphenicol</br> | 7. Pick 8 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of chloramphenicol</br> | ||
| Line 470: | Line 470: | ||
5. Link gene with terminator under 16℃ for 8 hours</br> | 5. Link gene with terminator under 16℃ for 8 hours</br> | ||
6. Transformation</br></p> | 6. Transformation</br></p> | ||
| − | <img style="width: | + | <img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/c/c1/Amoy-Notebook_node37-1.jpeg" /> |
<p class="detail_p"></br> | <p class="detail_p"></br> | ||
7. Pick 8 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of chloramphenicol</br> | 7. Pick 8 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of chloramphenicol</br> | ||
| Line 494: | Line 494: | ||
5. Link gene with terminator under 16℃ for 8 hours</br> | 5. Link gene with terminator under 16℃ for 8 hours</br> | ||
6. Transformation</br></p> | 6. Transformation</br></p> | ||
| − | <img style="width: | + | <img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/1/18/Amoy-Notebook_node38-1.jpeg" /> |
<p class="detail_p"></br> | <p class="detail_p"></br> | ||
7. Pick 8 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of chloramphenicol</br> | 7. Pick 8 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of chloramphenicol</br> | ||
| Line 514: | Line 514: | ||
1. Double enzyme digestion of LacI_B0032 and LeuDH_T</br> | 1. Double enzyme digestion of LacI_B0032 and LeuDH_T</br> | ||
2. Electrophoresis analysis of double digested result</br></p> | 2. Electrophoresis analysis of double digested result</br></p> | ||
| − | <img style="width: | + | <img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/a/aa/Amoy-Notebook_node21-1.jpeg" /> |
<p class="detail_p"></br> | <p class="detail_p"></br> | ||
3. Extract double digested product</br> | 3. Extract double digested product</br> | ||
| Line 520: | Line 520: | ||
5. Link gene with terminator under 16℃ for 8 hours</br> | 5. Link gene with terminator under 16℃ for 8 hours</br> | ||
6. Transformation</br></p> | 6. Transformation</br></p> | ||
| − | <img style="width: | + | <img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/c/c4/Amoy-Notebook_node21-2.jpeg" /> |
<p class="detail_p"></br> | <p class="detail_p"></br> | ||
7. Pick 8 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of chloramphenicol</br> | 7. Pick 8 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of chloramphenicol</br> | ||
| Line 540: | Line 540: | ||
1. Double enzyme digestion of LacI_B0032 and LeuDH_T</br> | 1. Double enzyme digestion of LacI_B0032 and LeuDH_T</br> | ||
2. Electrophoresis analysis of double digested result</br></p> | 2. Electrophoresis analysis of double digested result</br></p> | ||
| − | <img style="width: | + | <img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/1/1b/Amoy-Notebook_node22-1.jpeg" /> |
<p class="detail_p"></br> | <p class="detail_p"></br> | ||
3. Extract double digested product</br> | 3. Extract double digested product</br> | ||
| Line 546: | Line 546: | ||
5. Link gene with terminator under 16℃ for 8 hours</br> | 5. Link gene with terminator under 16℃ for 8 hours</br> | ||
6. Transformation</br></p> | 6. Transformation</br></p> | ||
| − | <img style="width: | + | <img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/7/70/Amoy-Notebook_node22-2.jpeg" /> |
<p class="detail_p"></br> | <p class="detail_p"></br> | ||
7. Pick 8 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of chloramphenicol</br> | 7. Pick 8 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of chloramphenicol</br> | ||
8. Extract the plasmids</br> | 8. Extract the plasmids</br> | ||
9. Electrophoresis analysis of plasmids</br></p> | 9. Electrophoresis analysis of plasmids</br></p> | ||
| − | <img style="width: | + | <img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/f/f9/Amoy-Notebook_node22-3.jpeg" /> |
<p class="detail_h1">Product:</br></p> | <p class="detail_h1">Product:</br></p> | ||
<p class="detail_p">isolated circuit with RBS_B0032 and gene_ldh</br></p> | <p class="detail_p">isolated circuit with RBS_B0032 and gene_ldh</br></p> | ||
| Line 567: | Line 567: | ||
1. Double enzyme digestion of LacI_B0032 and LeuDH_T</br> | 1. Double enzyme digestion of LacI_B0032 and LeuDH_T</br> | ||
2. Electrophoresis analysis of double digested result</br></p> | 2. Electrophoresis analysis of double digested result</br></p> | ||
| − | <img style="width: | + | <img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/4/45/Amoy-Notebook_node23-1.jpeg" /> |
<p class="detail_p"></br> | <p class="detail_p"></br> | ||
3. Extract double digested product</br> | 3. Extract double digested product</br> | ||
| Line 573: | Line 573: | ||
5. Link gene with terminator under 16℃ for 8 hours</br> | 5. Link gene with terminator under 16℃ for 8 hours</br> | ||
6. Transformation</br></p> | 6. Transformation</br></p> | ||
| − | <img style="width: | + | <img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/0/0e/Amoy-Notebook_node23-2.jpeg" /> |
<p class="detail_p"></br> | <p class="detail_p"></br> | ||
7. Pick 8 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of chloramphenicol</br> | 7. Pick 8 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of chloramphenicol</br> | ||
8. Extract the plasmids</br> | 8. Extract the plasmids</br> | ||
9. Electrophoresis analysis of plasmids</br></p> | 9. Electrophoresis analysis of plasmids</br></p> | ||
| − | <img style="width: | + | <img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/f/f7/Amoy-Notebook_node23-3.jpeg" /> |
<p class="detail_h1">Product:</br></p> | <p class="detail_h1">Product:</br></p> | ||
<p class="detail_p">isolated circuit with RBS_B0032 and gene_ldh</br></p> | <p class="detail_p">isolated circuit with RBS_B0032 and gene_ldh</br></p> | ||
| Line 594: | Line 594: | ||
1. Double enzyme digestion of LacI_B0032 and LeuDH_T</br> | 1. Double enzyme digestion of LacI_B0032 and LeuDH_T</br> | ||
2. Electrophoresis analysis of double digested result</br></p> | 2. Electrophoresis analysis of double digested result</br></p> | ||
| − | <img style="width: | + | <img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/8/87/Amoy-Notebook_Node41_figure1.jpg" /> |
<p class="detail_p"></br> | <p class="detail_p"></br> | ||
3. Extract double digested product</br> | 3. Extract double digested product</br> | ||
| Line 600: | Line 600: | ||
5. Link gene with terminator under 16℃ for 8 hours</br> | 5. Link gene with terminator under 16℃ for 8 hours</br> | ||
6. Transformation</br></p> | 6. Transformation</br></p> | ||
| − | <img style="width: | + | <img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/e/e7/Amoy-Notebook_node24-2.jpeg" /> |
<p class="detail_p"></br> | <p class="detail_p"></br> | ||
7. Pick 8 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of chloramphenicol</br> | 7. Pick 8 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of chloramphenicol</br> | ||
8. Extract the plasmids</br> | 8. Extract the plasmids</br> | ||
9. Electrophoresis analysis of plasmids</br></p> | 9. Electrophoresis analysis of plasmids</br></p> | ||
| − | <img style="width: | + | <img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/8/87/Amoy-Notebook_Node41_figure1.jpg" /> |
<p class="detail_h1">Product:</br></p> | <p class="detail_h1">Product:</br></p> | ||
<p class="detail_p">isolated circuit with RBS_B0032 and gene_ldh</br></p> | <p class="detail_p">isolated circuit with RBS_B0032 and gene_ldh</br></p> | ||
| Line 621: | Line 621: | ||
1. Double enzyme digestion of P<sub>lac</sub> and RBS_B0032</br> | 1. Double enzyme digestion of P<sub>lac</sub> and RBS_B0032</br> | ||
2. Electrophoresis analysis of double digested result of plasmid</br></p> | 2. Electrophoresis analysis of double digested result of plasmid</br></p> | ||
| − | <img style="width: | + | <img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/1/1f/Amoy-Notebook_Node32_figure1.jpg" /> |
<p class="detail_p"></br> | <p class="detail_p"></br> | ||
3. Extract double digested promoter LacI</br> | 3. Extract double digested promoter LacI</br> | ||
| Line 627: | Line 627: | ||
5. Link promoter with rbs under 16℃ for 8 hours</br> | 5. Link promoter with rbs under 16℃ for 8 hours</br> | ||
6. transformation</br></p> | 6. transformation</br></p> | ||
| − | <img style="width: | + | <img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/7/7a/Amoy-Notebook_node32-2.jpeg" /> |
<p class="detail_p"></br> | <p class="detail_p"></br> | ||
7. Pick 10 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of amp</br> | 7. Pick 10 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of amp</br> | ||
8. Extract the plasmids</br> | 8. Extract the plasmids</br> | ||
9. Electrophoresis analysis of plasmids</br></p> | 9. Electrophoresis analysis of plasmids</br></p> | ||
| − | <img style="width: | + | <img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/c/c9/Amoy-Notebook_Node32_figure3.jpg" /> |
<p class="detail_h1">Product:</br></p> | <p class="detail_h1">Product:</br></p> | ||
<p class="detail_p"> Plasmid of LacI linked with RBS_B0032</br></p> | <p class="detail_p"> Plasmid of LacI linked with RBS_B0032</br></p> | ||
| Line 653: | Line 653: | ||
4. Ligate under 16℃ for 8 hours</br> | 4. Ligate under 16℃ for 8 hours</br> | ||
5. Transformation</br></p> | 5. Transformation</br></p> | ||
| − | <img style="width: | + | <img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/e/ec/Amoy-Notebook_node11-2.jpeg" /> |
<p class="detail_p"></br> | <p class="detail_p"></br> | ||
6. Pick 8 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of chloramphenicol. Culture at 37℃,200rpm for 12~14 hours.</br> | 6. Pick 8 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of chloramphenicol. Culture at 37℃,200rpm for 12~14 hours.</br> | ||
| Line 680: | Line 680: | ||
4. Ligate under 16℃ for 8 hours</br> | 4. Ligate under 16℃ for 8 hours</br> | ||
5. Transformation</br></p> | 5. Transformation</br></p> | ||
| − | <img style="width: | + | <img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/0/01/Amoy-Notebook_node12-2.jpeg" /> |
<p class="detail_p"></br> | <p class="detail_p"></br> | ||
6. Pick 8 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of chloramphenicol. Culture at 37℃,200rpm for 12~14 hours.</br> | 6. Pick 8 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of chloramphenicol. Culture at 37℃,200rpm for 12~14 hours.</br> | ||
| Line 709: | Line 709: | ||
4. Ligate under 16℃ for 8 hours</br> | 4. Ligate under 16℃ for 8 hours</br> | ||
5. Transformation</br></p> | 5. Transformation</br></p> | ||
| − | <img style="width: | + | <img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/1/1f/Amoy-Notebook_node13-2.jpeg" /> |
<p class="detail_p"></br> | <p class="detail_p"></br> | ||
6. Pick 8 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of chloramphenicol. Culture at 37℃,200rpm for 12~14 hours.</br> | 6. Pick 8 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of chloramphenicol. Culture at 37℃,200rpm for 12~14 hours.</br> | ||
| Line 733: | Line 733: | ||
1. Add 20ul ddH20 to solve the dry powder</br> | 1. Add 20ul ddH20 to solve the dry powder</br> | ||
2. Suck 10ul of plasmid into 50ul of competent cell for transformation</br></p> | 2. Suck 10ul of plasmid into 50ul of competent cell for transformation</br></p> | ||
| − | <img style="width: | + | <img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/8/87/Amoy-Notebook_Node41_figure1.jpg" /> |
<p class="detail_p"></br> | <p class="detail_p"></br> | ||
3. Pick a single colony from the agar plate using a sterile pipette tip. </br> | 3. Pick a single colony from the agar plate using a sterile pipette tip. </br> | ||
| Line 753: | Line 753: | ||
1. Add 20ul ddH20 to solve the dry powde</br> | 1. Add 20ul ddH20 to solve the dry powde</br> | ||
2. Suck 10ul of plasmid into 50ul of competent cell for transformation</br></p> | 2. Suck 10ul of plasmid into 50ul of competent cell for transformation</br></p> | ||
| − | <img style="width: | + | <img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/8/87/Amoy-Notebook_Node41_figure1.jpg" /> |
<p class="detail_p"></br> | <p class="detail_p"></br> | ||
3. Pick a single colony from the agar plate using a sterile pipette tip. </br> | 3. Pick a single colony from the agar plate using a sterile pipette tip. </br> | ||
| Line 775: | Line 775: | ||
3. Link promoter with rbs under 16℃ for 8 hours</br> | 3. Link promoter with rbs under 16℃ for 8 hours</br> | ||
4. Transformation</br></p> | 4. Transformation</br></p> | ||
| − | <img style="width: | + | <img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/1/18/Amoy-Notebook_node31-1.jpeg" /> |
<p class="detail_p"></br> | <p class="detail_p"></br> | ||
5. Pick 10 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of amp</br> | 5. Pick 10 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of amp</br> | ||
Revision as of 10:05, 18 September 2015
NOTEBOOK
Initially, they used isolated enzymes, which can be disadvantageous for the reason that enzymes are always destabilized in the isolation and purification process. What's more, the cofactor-NADH is rather an expensive raw material, which will enhance the cost of L-tert-leucine production. So scientists introduced whole-cell biocatalysts to L-tert-leucine production. Whole-cell biocatalysts could stabilize enzymes and reduce the addition level of cofactor NADH. In the path of building our biobricks, we divided the circuits into two modules. One is promoter linked with rbs and the other is gene linked with terminator. The dendrogram below is our experiments detail. Click each bottom for more information.
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