Team:Warsaw/Calendar-Main/22 September 2008
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<h3>'Hunter and prey' system tests: Competition tests</h3> | <h3>'Hunter and prey' system tests: Competition tests</h3> | ||
<h4>Weronika</h4> | <h4>Weronika</h4> | ||
- | <p><ol><li>Plasmid isolation from 19 September cultures.</li><li>Digest with SacI and BamHI.</li><li>Electrophoresis.</li></ol></p> | + | <p><ol><li>Plasmid <a href=https://2008.igem.org/wiki/index.php?title=Wiki/Team:Warsaw/protocols#plasmid_DNA_isolation>isolation</a> from 19 September cultures.</li><li>Digest with SacI and BamHI.</li><li>Electrophoresis.</li></ol></p> |
[photo of the gel is to be placed here] | [photo of the gel is to be placed here] |
Revision as of 18:29, 27 October 2008
MutD5 testingPiotrInoculation of MutD5 carrying: pACYC177+OmpA_Z_alpha, pACYC177+OmpA_Z_omega, pACYC177+Omp_A_omega and pACYC177+OmpA_omega_ΔA + induction using 0.25mM IPTG. 'Hunter and prey' system tests: Competition testsWeronika
Conclusion: cells with interacting protein survive competition! Mutagenesis of protein APawełMutagenesis of protein A was performed using 2 pairs of primers: ADelL+KpnI and ADelP (deletion of aminoacids involved in interaction with protein Z) and AMutL+KpnI and AMutP (changing of few aminoacids involved in interaction with protein Z). Mutagenesis was performed on 3 vectors: pACYClac+ompA-ΔA-omega, pACYClac+ompa-ΔA-alpha and pACYClac+ ompa-omega-ΔA. Each mutagenesis was performed using each primer at final concentration 0.1 μM, dNTPs at final concentration 0.25 μM and Walk (Pfu) polymerase (shipped by A&A Biotechnology), with 100 ng of DNA template.
94°C 5 min 94°C 30 s 55°C 30 s 72°C 10 min 72°C 8 min 4°C hold Preparation of ΔA (BBa_K103003)Michał K.Inoculation of only one colony which grown from transformation (19 September) - pSB1A3+ΔAplasmid into liquid LB + ampicillin.
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