Team:UTP-Panama/Week 16
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==September 19== | ==September 19== | ||
===WET LAB=== | ===WET LAB=== | ||
+ | ====I. DIGESTION==== | ||
For each Eppendorf PCR was added the following:<br> | For each Eppendorf PCR was added the following:<br> | ||
1. 10µL DNA (residue of mini prep)<br> | 1. 10µL DNA (residue of mini prep)<br> | ||
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Note: Make sure to mix all the components in the centrifuge <br> | Note: Make sure to mix all the components in the centrifuge <br> | ||
- | 7. 2 eppendorf tubes were incubated in the thermocycler during 1 hour at 37°C : <br> | + | 7. Two (2)eppendorf tubes were incubated in the thermocycler during 1 hour at 37°C : <br> |
a. UPSTREAM (GaTech) <br> | a. UPSTREAM (GaTech) <br> | ||
b. DOWNSTREAM (Bristol)<br> | b. DOWNSTREAM (Bristol)<br> | ||
8. Once again, tubes were incubated in the thermocycler during 20 minutes at 80°C<br> | 8. Once again, tubes were incubated in the thermocycler during 20 minutes at 80°C<br> | ||
9. We stored at -20°C until it is used for ligation.<br> | 9. We stored at -20°C until it is used for ligation.<br> | ||
+ | |||
+ | ==== Transformation of Competent Cells==== | ||
+ | A. | ||
+ | 4 petri dishes were filled with 5mL of solid LB | ||
+ | 3 positive controls and 1 negative control. | ||
+ | [[File:calculo 19sept.jpg]] | ||
+ | |||
+ | Total: '''19.36µL para 20µL de LB'''<br> | ||
+ | |||
+ | ''''Content of controls:'''' <br> | ||
+ | Positive Control: 50µL competent cells + 2µL BBa_K410000 is resuspended.<br> | ||
+ | Negative Control: 50µL competent cells <br> | ||
+ | |||
+ | 1. In 3 eppendorf tubes was added the specified amount in positive control and were resuspended.<br> | ||
+ | 2. Tubes in previous step remained settled in ice during 30 minutes.<br> | ||
+ | 3. Afterwards, cold shock carried out, the 4 eppendorf are set in water bath for a minute. (T=42°C)<br> | ||
+ | 4. Right after the water bath, it remained in ice during 5 minutes.<br> | ||
+ | 5. Added 200µL cold SOC to each eppendorf tube, then resuspended<br> | ||
+ | 6. Every petri dish was sealed with parafilm and was appropriately labeled; afterwards they were put in the incubator<br> | ||
==September 20== | ==September 20== | ||
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Future projects | Future projects | ||
- | ===WET LAB=== | + | ====WET LAB==== |
- | + | ||
- | -- | + | |
+ | Objetives or Title:<br> | ||
+ | In the picture of the result of the electrophoresis of Biobrick BBa-K381001, neither the patron nor the plasmids could be observed, for this reason the protocol was repeated the next day.<br> | ||
+ | 1 2 3 4 | ||
+ | [[File:igem utp 20-09-2011.jpg]] | ||
+ | |||
+ | 1, 2 : BBa_K381001 (positive control) | ||
+ | |||
+ | 3, 4 : BBa_K381001 (negative control) | ||
==September 21== | ==September 21== | ||
===WET LAB=== | ===WET LAB=== | ||
- | + | [[File:3CONTROLES 21SEPT CONTRASTE INVERTIDO Bristol.jpg]] | |
- | + | ||
- | + | This day the electrophoresis test was performed to the obtained plasmids with BBa-K381001 in Sept 14, 2011.<br> | |
- | + | Also were transformed competent cells with BBa-K672000 (RENBO); Sept 21, 2011.<br> | |
- | ( | + | |
- | + | ||
==September 23== | ==September 23== | ||
===WET LAB=== | ===WET LAB=== | ||
- | + | We carried out a '''dirty mini prep protocol''' to BBa-K672000 to send 250ng DNA in 10µL TE. A sample was preserved for electrophoresis. | |
- | - | + | |
- | DNA | + | |
==September 24== | ==September 24== | ||
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===GENERAL SESSION === | ===GENERAL SESSION === | ||
Afternoon: Talikng about WET LAB final activities. | Afternoon: Talikng about WET LAB final activities. | ||
- | Design of the '''"SB UTP 1.0"''' and '''"SB UTP Project 1.0"''' | + | Design of the '''"SB UTP 1.0"''' and '''"SB UTP Project 1.0"'''<br> |
Discussion about remake the experiments with the Bristol and Gatech Biobricks (experience). | Discussion about remake the experiments with the Bristol and Gatech Biobricks (experience). | ||
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Latest revision as of 05:00, 29 September 2011
Home |
Week 1 | Week 2 | Week 3 | Week 4 | Week 5 | Week 6 | Week 7 | Week 8 | Week 9 | Week 10 | Week 11 | Week 12 | Week 13 | Week 14 | Week 15 | Week 16 | Week 17 | After Regional Week 1 | After Regional Week 2 | Week 16: September 19 to 24September 19WET LABI. DIGESTIONFor each Eppendorf PCR was added the following: There was added the 6 components to the small tube of PCR. 7. Two (2)eppendorf tubes were incubated in the thermocycler during 1 hour at 37°C : Transformation of Competent CellsA. 4 petri dishes were filled with 5mL of solid LB 3 positive controls and 1 negative control. Total: 19.36µL para 20µL de LB 'Content of controls:' 1. In 3 eppendorf tubes was added the specified amount in positive control and were resuspended. September 20Scientific Comunication ActivitiesTree sessions: WET LABObjetives or Title: 1 2 3 4 1, 2 : BBa_K381001 (positive control) 3, 4 : BBa_K381001 (negative control) September 21WET LABThis day the electrophoresis test was performed to the obtained plasmids with BBa-K381001 in Sept 14, 2011. September 23WET LABWe carried out a dirty mini prep protocol to BBa-K672000 to send 250ng DNA in 10µL TE. A sample was preserved for electrophoresis. September 24GENERAL SESSIONAfternoon: Talikng about WET LAB final activities.
Design of the "SB UTP 1.0" and "SB UTP Project 1.0" |