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Team:Chiba/Assay/store
From 2013.igem.org
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<br><b>Detailed procedure</b> | <br><b>Detailed procedure</b> | ||
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| - | + | 1. E. coli strain BL21 and SHuffle® were transformed with the plasmids shown in Fig. 1. | |
| - | <br>2.All transformants were inoculated into small (2 mL) culture and was shaken for 12h (at 37°C). | + | <br> |
| - | <br>3.Inoculated into flesh media (2 mL), shaken for 3 hours. | + | 2. All transformants were inoculated into small (2 mL) culture and was shaken for 12h (at 37°C). |
| - | <br>4.We added L-arabinose into each sample (final conc. 0.2%). Then cultured for another 9 hours (at 37°C). | + | <br> |
| - | <br>5.After 9 hours, we measured cell density (OD600) of every sample, and put 10^7 cell of E.coli to fresh medium containing various concentration of iron citrate or iron ascorbate. | + | 3. Inoculated into flesh media (2 mL), shaken for 3 hours. |
| - | <br>6.Then we shaking cultured E.coli for 12 hours. | + | <br> |
| - | <br>7.We got 1 mL aliquot from each sample and centrifuged with 7,000 rpm, at 25℃ for 2 minutes. | + | 4. We added L-arabinose into each sample (final conc. 0.2%). Then cultured for another 9 hours (at 37°C). |
| - | <br>8.We wasted supernatant and resuspended with 1 mL saline solution (0.9% NaClaq), and we measured cell density (OD600). | + | <br> |
| - | <br>9.5 | + | 5. After 9 hours, we measured cell density (OD600) of every sample, and put 10^7 cell of E.coli to fresh medium containing various concentration of iron citrate or iron ascorbate. |
| - | <br><br> | + | <br> |
| + | 6. Then we shaking cultured E.coli for 12 hours. | ||
| + | <br> | ||
| + | 7. We got 1 mL aliquot from each sample and centrifuged with 7,000 rpm, at 25℃ for 2 minutes. | ||
| + | <br> | ||
| + | 8. We wasted supernatant and resuspended with 1 mL saline solution (0.9% NaClaq), and we measured cell density (OD600). | ||
| + | <br> | ||
| + | 9. 5 μl of the diluted cell suspension was spotted on the LB agar medium and incubated for 12 hours. Approximately 107, 106, 105, 104, 103, and 102 cells were contained in the spots. | ||
| + | |||
| + | |||
| + | <br><br> | ||
Revision as of 09:14, 27 September 2013
Storage実験方法
Experiment:
We constructed two plasmids as shown in Fig. 1. Human ferritin genes (fth1 and ftl) are placed on the high-copy plasmid under the control of BAD promoter. By adding arabinose into the media, Human ferritin proteins are induced.E. coli strain BL21 and SHuffle® (要link) were transformed with above plasmids. The resultant “ferritin generators” were cultured in the presence of iron citrate (Fe3+) or iron ascorbate (Fe2+), and checked final cell density and colony forming efficiency. As a control, we conducted the same experiment with “sfgfp generator”.
Detailed procedure
1. E. coli strain BL21 and SHuffle® were transformed with the plasmids shown in Fig. 1.
2. All transformants were inoculated into small (2 mL) culture and was shaken for 12h (at 37°C).
3. Inoculated into flesh media (2 mL), shaken for 3 hours.
4. We added L-arabinose into each sample (final conc. 0.2%). Then cultured for another 9 hours (at 37°C).
5. After 9 hours, we measured cell density (OD600) of every sample, and put 10^7 cell of E.coli to fresh medium containing various concentration of iron citrate or iron ascorbate.
6. Then we shaking cultured E.coli for 12 hours.
7. We got 1 mL aliquot from each sample and centrifuged with 7,000 rpm, at 25℃ for 2 minutes.
8. We wasted supernatant and resuspended with 1 mL saline solution (0.9% NaClaq), and we measured cell density (OD600).
9. 5 μl of the diluted cell suspension was spotted on the LB agar medium and incubated for 12 hours. Approximately 107, 106, 105, 104, 103, and 102 cells were contained in the spots.
