Team:TU-Delft/Project/Transportation
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In site-directed mutagenesis we introduced two stop codons in the coding sequence of the Sec-peptide to prevent this part from being transcribed an translated. A start codon was present shortly after the location of the newly introduced stop codons. Since the sequence is very close to the promotor translation of the parts afterwards, this sequence should still function properly. This is not certain however, and so we had a more elaborate second approach. This involved using PCR to get the coding sequence before and, separately, after the Sec-peptide. Paying attention to the reading frame, we digest and ligate these sequences to have once again a coding sequence analogous to the original one, but without the Sec-peptide sequence. This led to a construct which contained in sequential order the p-BAD promotor, Mfp-5, GFP and OmpA. | In site-directed mutagenesis we introduced two stop codons in the coding sequence of the Sec-peptide to prevent this part from being transcribed an translated. A start codon was present shortly after the location of the newly introduced stop codons. Since the sequence is very close to the promotor translation of the parts afterwards, this sequence should still function properly. This is not certain however, and so we had a more elaborate second approach. This involved using PCR to get the coding sequence before and, separately, after the Sec-peptide. Paying attention to the reading frame, we digest and ligate these sequences to have once again a coding sequence analogous to the original one, but without the Sec-peptide sequence. This led to a construct which contained in sequential order the p-BAD promotor, Mfp-5, GFP and OmpA. | ||
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{{TU-footer}} | {{TU-footer}} |
Revision as of 20:21, 21 September 2011