From 2008.igem.org
Objectives
- Convert GFP (BBa_E0040) into a fusion brick using site-directed mutagenesis.
- Convert pRL1383a into a Biobrick vector by replacing its natural MCS with the Biobrick MCS
Protocol
PCR mutagenesis of GFP
- 1 μl colony sample (above)
- 0.5 μl 10mM forward primer
- 0.5 μl 10mM reverse primer
- 3 μl nanopure water
- 5 μl Taq (we used EconoTaq Green Taq)
- Ran for 30 cycles of denaturing, annealing, extension
- Initial denature @ 94C for 2 min.
- Denature @ 94C for 30 sec.
- Anneal @ 55C for 30 sec.
- Extend @ 72C for 60 sec.
- Final extension @ 72C for 10 min.
- Held @ 4C inifinitly.
GFP fusion brick (site directed mutagenesis)
| Primer
| Sequence
| Length
| G/C content
| Tm
| Notes
|
| GFP fusion foward
| GCCGCTTCTAGAcgtaaaggag
| 22 bp
| 54.55%
| 60.2 C
| PCR out from E0040, starts annealing from partial NotI (5 of 8 nucleotides of) site, continues with XbaI, omits TG of ATG codon for site directed mutagenesis, begins again with GFP codon 2-4 (cgt aaa gga)
|
| GFP fusion reverse
| cgagtcagtgagcgaggaag
| 20 bp
| 60%
| 59.6 C
| PCR out from E0040, priming after all end sites (5'taataa t actagt a gcggccg ctgcag gCTTCCTCGCTCACTGACTCG3')
|
Subcloning of GFP fusion brick and pRL1383a Biobrick vector
Results
Discussion
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