Insert design flowchart. See Section 12 for a detailed discussion.

DNA Vaccine Vector production and use flowchart.

Antibiotic Free Bird Flu DNA vaccine vector. Vector specific features such as the CMV-HTLV-1 R-U5 derived mRNA leader (UTR) chimeric SV40-CMV promoter, and RNA selectable marker are indicated.

A. Inducible fed-batch plasmid production fermentation process. B. E. coli strain DH5α + pNTCUltra1 plasmid inducible fed-batch fermentation growth and plasmid yield profiles. Fermentation was shifted from 30 to 42°C at 29hrs to induce plasmid production, plasmid yield reached 2130 mg/L.

A. Annotated pDNAVACCUltra-1 (pNTCUltra-1) restriction map. Critical features such as the mRNA leader (UTR), chimeric SV40-CMV promoter, kanR gene, and functional domains in the origin (PAS-BL, RNAII promoter, RNase H cleavage site) are indicated. This vector targets a fusion antigen (antigens 1 and 2) for proteosomal degradation by fusion to the C-terminus of Ubiquitin A76. B. Plasmid DNA replication. For the leading strand, a RNA polymerase transcript (RNAII) either forms a replication driving R-loop (RNA:DNA hybrid) with the origin (left) or a nonproductive interaction with the antisense RNAI copy number regulator (right). The R-loop is cleaved by RNase H, the resulting 3′ OH serving as a primer for DNA pol I DNA synthesis. Replication of the leading strand exposes a phiX174 type primosome assembly site on the lagging strand (PAS-BL), which binds primosomal proteins (see Section 4.1). Lagging strand replication initiated at PAS-BL terminates at a termination site (ter) within the origin. Leading strand replication proceeds around the plasmid, also stopping at the ter site. DNA Pol I and DNA ligase are required after Pol III mediated leading and lagging strand replication to remove primers and seal nicks, respectively. DNA gyrase then negatively supercoils the resultant covalently closed circular (CCC) plasmid.