Team:Bilkent UNAM Turkey/Experiment
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<tr><th>Nucleic Acid Conc.</th> <th>Unit</th><th>A260</th><th>A280</th><th>260/280</th><th>260/230</th><th>Sample Type</th> | <tr><th>Nucleic Acid Conc.</th> <th>Unit</th><th>A260</th><th>A280</th><th>260/280</th><th>260/230</th><th>Sample Type</th> | ||
<tr><td>361.4</td><td>ng/µl</td><td>7.228</td><td>4.334</td><td>1.67</td><td>1.82</td><td>DNA</td> | <tr><td>361.4</td><td>ng/µl</td><td>7.228</td><td>4.334</td><td>1.67</td><td>1.82</td><td>DNA</td> | ||
- | <tr>384.9 ng/µl 7.698 4.554 1.69 1.82 DNA | + | <tr><td>384.9<td> ng/µl<td> 7.698<td> 4.554<td> 1.69<td> 1.82<td> DNA |
- | <tr>558.7 ng/µl 11.174 7.232 1.55 1.65 DNA | + | <tr><td>558.7<td> ng/µl<td> 11.174<td> 7.232<td> 1.55<td> 1.65<td> DNA |
- | + | </table> | |
We proceeded to transformation of this plasmids to microalgae. We co-transformed Chlamydomonas reinhardtii to Tris-acetate-phosphate plus neomycine agar plates with pRbcnfsI and pKS-aphVIII-lox plasmid in order to select colonies based on the arginine deficiency in mutant strain cc-425 of Chlamydomonas reinhardtii. Next step was to collect colonies from plate. But due to time constraints we could not obtain colonies from this experiment yet. After collecting colonies, we plan to subculture colonies in the presence of trinitrotoluene (TNT) and check for change in its concentration.<br> | We proceeded to transformation of this plasmids to microalgae. We co-transformed Chlamydomonas reinhardtii to Tris-acetate-phosphate plus neomycine agar plates with pRbcnfsI and pKS-aphVIII-lox plasmid in order to select colonies based on the arginine deficiency in mutant strain cc-425 of Chlamydomonas reinhardtii. Next step was to collect colonies from plate. But due to time constraints we could not obtain colonies from this experiment yet. After collecting colonies, we plan to subculture colonies in the presence of trinitrotoluene (TNT) and check for change in its concentration.<br> | ||
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