Team:DTU-Denmark/Notebook/2 August 2013
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*PCR of Nir, His-Tag Sec, His-Tag TAT | *PCR of Nir, His-Tag Sec, His-Tag TAT | ||
*Miniprep re-purification with columns | *Miniprep re-purification with columns | ||
+ | *Inoculation of samples for mini prep | ||
==Who was in the lab== | ==Who was in the lab== |
Revision as of 16:39, 2 August 2013
2 August 2013
Contents |
lab 208
Main purpose
- Gel purification of Cyc and Nir
- USER reaction
- PCR of Nir, His-Tag Sec, His-Tag TAT
- Miniprep re-purification with columns
- Inoculation of samples for mini prep
Who was in the lab
Gosia, Kristian, Natalia, Julia
Procedure
Gel purification
- Gel purification was performed according to protocol included in QIAEX, Gel Extraction Kit.
USER reaction
- USER reaction was performed according to standard protocol SOP1. We use DNA linear fragment containing pZA21 bacbone,cycAX with His-Tag sequence.
PCR
- PCR according to standard PCR protocol.
Samples names:
- 1,2 - Nir 48 (primers 48a, 48b) on template of Nir (too long fragment amplified at the beginning of work with Nir PCR)
- 3,4 - Sec His-Tag, primers 19a, 19b; template: Sec 2
- 5,6 - Tat His-Tag, primers 20a, 20b; template: TAT 2 1
- 7,8 - Tat His-Tag, primers 20a, 20b; template: TAT 3 2
- 9, 10 - Tat His-Tag, primers 20a, 20b; template: TAT 3 1a
- 11, 12, 13 - negative controls as follows for: Tat His-Tag, Nir, Sec His-Tag
- Program for samples: 1,2,12 - Program for Nir on Eppendorf machine
- 3,4,13 - 10 cycles 58.5 C annealing, 1 min elongation and 25 cycles on 67 C annealing
- 5-11 - 10 cycles on 54.5 C annealing and 25 cycles on 64 C annealing
Purification of plasmids after ethanol purification
According to protocol attached to the DNA purification kit, QIAGEN
Results
Conclusion
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