The p DOM vaccine construct (Fig 1) has been described previousl

The p.DOM vaccine construct (Fig. 1) has been described previously 26. The construct encodes the first domain, DOM, of FrC from TT (TT865–1120) covalently fused to an N-terminal VH leader of the IgM from the mouse BCL1 lymphoma. The p.DOM-PSMA27, pDOM-PSMA663, and pDOM-PSMA711 vaccines encode the PSMA27, PSMA663, and PSMA711 HLA-A*0201-binding epitopes fused to the C-terminus of DOM. They were created by amplification of the p.DOM vaccine insert by PCR with the F1 forward primer and a reverse primer encoding the epitope; R1, R2, and R3 for PSMA27, PSMA663, and PSMA711 respectively. Primer sequences are listed in Table 1. The full-length human PSMA vaccines which encode the full-length protein (750 residues in total; 1–19 intracellular,

PR-171 concentration 20–44 transmembrane

and 45–750 extracellular) were created by PCR using human prostate cDNA generated from total RNA (Clontech) with the Superscript First-Strand cDNA Synthesis kit (Invitrogen, Paisley, UK) as a template. The F2 and R4 primers were used to amplify the full-length PSMA sequence. The PSMA gene was fused to the leader sequence in two steps. The first fragment was made using the p.DOM construct as a template with the F1 primer and the R5 reverse AZD9668 primer, resulting in a BCL1 fragment with a PSMA overhang. The second fragment was generated by PCR using the PSMA cDNA as a template, F3 and R6 primers, resulting in a PSMA fragment with a BCL1 overhang upstream. These two DNA fragments were joined using the primers F1 and R6. This fragment was modified using the F4 and R7 primers to incorporate restriction sites. To allow fusion of the DOM sequence to PSMA, the BCL1-PSMA DNA fragment was also modified, using the F1 and R8 primers. ADP ribosylation factor Purified PCR products were digested and inserted between the HindIII (or BamHI for p.PSMA) and NotI restriction sites in the pcDNA3.1 plasmid (Invitrogen). In the case of the p.PSMA-DOM construct, the digested PCR product was inserted between HindIII and NotI restriction sites upstream of the DOM sequence in a modified version of pcDNA3.1.

Vaccines were prepared and verified as described previously 50. The ability of the DNA vaccines to prime PSMA peptide-specific CD8+ T cells in individual HHD mice was assessed ex vivo using an IFN-γ ELISpot assay (BD ELISpot Set, BD Pharmingen, San Diego, CA). Briefly, viable mononuclear cells from individual splenocyte preparations were isolated by density gradient centrifugation. Cells (2×105 cells/well) were incubated in complete medium for 24 h with the corresponding PSMA HLA-A*0201 peptide (10−6–10−9 M) to assess CD8+ T-cell responses or with the p30 peptide (10−6 M) to evaluate CD4+ T-cell responses. Control wells were incubated without peptide to assess background. Samples were plated in triplicate and the mean of the readings is expressed as SFCs per million (106) cells. To assess avidity, the number of SFC/106 cells at the peptide concentration inducing the greatest response was assigned a value of 100%.

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