Part:BBa_K563001:Design

pDAL7(malate synthase promoter)

Design Notes

In order to determine the appropriate assembly standard which the part can be used with, it's necessary to check the sequence for each of the restriction enzymes. Sequence scanning of pDAL7 show that no EcoRI XhoI XbaI SpeI NcoI PstI BamHI exists. As our target gene comes from yeast and contains common restriction sites like EcoRI, NotI and SpeI, the stantard BioBrick prefix and suffix is no longer appropriate. Furthermore, the size of 7800bp makes it pretty expensive and inconvenient for chemical synthesis and codon optimization to avoid certain restriction sites. To match with the operation of downstream gene, the promoter parts also give up standard prefix and suffix. However, based on the modified plasmid backbone pSB1A11, we bring in some other common restriction sites, which also render functionality and ease-of-use of promoter parts.

Source

We isolate the sequece by PCR on Saccharomyces cerevisiae strain BY4742. For standard operation of BioBricks and easy-use for other teams, we add restriction sites at upstream and downstream of the sequence ( NcoI and XhoI respectively) by designing specific primers (details in sequence and feature annotations). Forward Primer(with restriction site and protective bases): (TCATGCCATGG)TACCTGGCATGCGCCCATGATAGTAC Reverse Primer(with restriction site and protective bases): (ATCCGCTCGAG)TGTTCAGTGCTCTTTACCGTGCCTAT

References

Identi¢cation of direct and indirect targets of theGln3 andGat1 activators by transcriptional pro¢ling in response to nitrogen availability in the short and long term. Bart Scherens, Andr´e Feller, Fabienne Vierendeels, Francine Messenguy & Evelyne Dubois. FEMS Yeast Res 6 (2006) 777–791.