Fig. 4. Therapeutic transgenes in the oFV backbone are stable for up to 3 in vitro passages, TK cDNA appears to be more stable than iCasp9 cDNA in the oFV backbone during in vivo amplification.

A oFV-TK and oFV-iCasp9 were serially passaged five times at a fixed MOI = 0.5 in U251-U3-mCherry-U3-luc cells and at the end of each passage (day 8 postinfection) the genomic DNA was isolated from the infected cells for a PCR amplification of the bel2 region (containing the transgene) or env (control). B., D. U251-U3-mCherry-U3-luc tumors from mice infected with oFV-TK/oFV-iCasp9 and treated with GCV (n = 3)/AP20187 (n = 2) or PBS control (n = 3 for oFV-TK and n = 2 for oFV-iCasp9) were explanted and cultured in vitro, then genomic DNA was isolated from the explants and PCR analyzed for the presence of the oFV-TK (B) or oFV-iCasp9 (D) provirus (env) as well as the intact transgene cDNA (bel2 region), C. qPCR reaction was performed on the DNA isolated from oFV-TK infected tumors to determine the env and TK copy number, result is normalized to endogenous β-actin copy number. +c – positive control (oFV-TK or –iCasp9 infectious clone DNA), -C – negative control (genomic DNA from uninfected U251-U3-mCherry-luc cells), NTC- no template control, P1-P5 – passage number, i-iv – specific tumors collected from the treated mice for analysis.