Gene Design

CLD G-Block

Modifications

CLD±

Thorell determined that the gene was capable of converting ClO2 to O2 and Cl- and that its activity was localized to the periplasm, even though its putative signal peptide had not been cleaved. In light of their results we decided to design a Cld gene (Cld SP+) where the putative signal peptide was replaced with the MalE signal peptide from E. coli that has been previously shown to be a superior signal for periplasmic localization that is cleaved (Samant et al. 2014). In addition we designed a Cld gene that lacked the signal sequence (Cld SP-) as a negative control.

Terminal Histidine Tag

In the event that the production of O2 from living cells proved inefficient, a C-terminal histidine tag was appended to both the CLD- and CLD+ G-Blocks in anticipation for the purification the expressed enzymes. Nickel Column info and reference pls.

Restriction Sites and Silent Mutation

Flanking these BsaI sites were XbaI (5’) and the BBa_ std 1 suffix (3’) to facilitate parts creation for the registry. WE note that the natural coding sequence contained none of the standard BBa_10 restrictions sites, but did contain a single internal BsaI site which we eliminated with a single base silent substitution (Fig_)

IDT Synthesis

Upon the finalization of our CLD G-Block designs, we were able to get the gene synthesized by IDT who was offering iGEM teams 15 000 base pairs worth of DNA for free.