A clinical grade high-titer PG13 clone expressing the 1928z chimeric antigen receptor (CAR) was generated by transiently transfecting Phoenix-eco cells with the plasmid encoding the gammaretroviral vector SFG-1928z12 (link) and subsequently infecting PG13 cells with cell-free vector stocks from the transfected Phoenix-eco cells. The PG13-1928z cell population was subsequently subcloned by limiting dilution. Clones were isolated and titers were determined by infecting HeLa cells under standardized conditions. High titer clones were identified by fluorescence activated cell sorting (FACS) using the anti-1928z CAR hamster monoclonal antibody 19E3 that was generated in-house by the MSKCC monoclonal antibody core facility. The high titer PG13-1928z clone 34 was subjected to a second round of subcloning by limiting dilution. The subclone PG13-1928z cl.3 was demonstrated to express the 19-28zCAR and was selected for its ability to efficiently transduce peripheral blood mononuclear cells (PBMCs). Integrity of the retroviral vector construct was demonstrated and a single copy of the integrated proviral vector was detected by Southern blot analysis in the genomic DNA extracted from PG13-1928z clone 3 (data not shown). The PG13-1928z clone 3 was expanded to generate a seed bank (SB) that was tested for absence of mycoplasm, replication competent retrovirus (RCR), and for sterility. The SB passed all required tests.