Hrp conjugated anti mouse igg each isotype antibody

To measure the epitope peptide-specific antibody titer, 96-well immunoplates (Thermo Fisher Scientific Co.) were coated with 5 μg/well of the MERS-CoV Spike-492 or Spike-492 (L506F) peptides. The mice sera were obtained by retro orbital bleeding and analyzed as previously described (22 (link)). To identify the isotype of the monoclonal antibody, the HRP-conjugated anti-mouse IgG (each isotype) antibody (Southern Biotechnology Associates Inc.) was used. For detection of cross-reactivity, 96-well immunoplates were coated with the MERS-CoV Spike-492 or Spike-492 (L506F) peptides and incubated with either 492-1G10E4E2 or 506-2G10G5 monoclonal antibody for 2 h before incubation with the secondary antibody. The absorbance was evaluated with the Spectra Max 250 microplate reader (Molecular Devices Co.) at 450 nm and then calculated with the SigmaPlot program to determine the affinity constant (EC50 value) as described previously (17 (link)).