Plan for the construction of E. coli vector pYPKa_E_FBA1tp
PCR with primers pfw630 & prv630 and template FBA1_template results in a 643bp PCR product
Primers annealing on template:
5ATAACAATACTGACAGTACTAAATAAT...ATAACCAAGTAATACATATTCAAA3
|||||||||||||||||||||||| tm 44.2 (dbd) 54.6
3TATTGGTTCATTATGTATAAGTTTaattaat5
5ttaaatATAACAATACTGACAGTACTAAATAAT3
||||||||||||||||||||||||||| tm 47.0 (dbd) 54.0
3TATTGTTATGACTGTCATGATTTATTA...TATTGGTTCATTATGTATAAGTTT5
Suggested PCR programs for Taq polymerase and for Polymerases with DNA binding domain:
Taq (rate 30 nt/s)
Three-step| 30 cycles | |SantaLucia 1998
94.0°C |94.0°C | |SaltC 50mM
__________|_____ 72.0°C |72.0°C|
04min00s |30s \ ________|______|
| \ 50.0°C/ 0min19s|10min |
| \_____/ | |
| 30s | |4-8°C
Pfu-Sso7d (rate 15s/kb)
Three-step| 30 cycles | |Breslauer1986,SantaLucia1998
98.0°C |98.0°C | |SaltC 50mM
__________|_____ 72.0°C |72.0°C|Primer1C 1µM
00min30s |10s \ 57.0°C ________|______|Primer2C 1µM
| \______/ 0min 9s|10min |
| 10s | |4-8°C
Clone the PCR product in pYPKa digested with EcoRV resulting in pYPKa_E_FBA1tp
Confirm the structure of the pYPKa_E_FBA1tp using primers 568, 342 and pfw630 in a multiplex PCR reaction.
Expected PCR products sizes from 568, 342 and pfw630 (bp):
pYPKa with insert in correct orientation: 1359, 1328
pYPKa with insert in reverse orientation: 1359, 674
Empty pYPKa clone : 716