The protocol is identical to the new ELISpot protocol described above (see Section 2.4.2) except for two steps. Firstly, instead of using antigen for coating, wells were coated with capture mAbs. Secondly, instead of using detection mAbs, a biotinylated antigen was used for detection. For the biotinylation of antigen, biotin ester (Surelink™ Chromophoric Biotin; VWR, Stockholm, Sweden)
dissolved in dimethylformamide (DMF) to 20 mg/ml was Veliparib added to DT or TTd in PBS (3–4 mg/ml) at a 10 times molar excess. The conjugates were incubated for 2 h at 25 °C at 400 rpm. The biotinylated antigens were dialyzed for 4 days against PBS at 4 °C using a 10 kDa cut off dialysis tube. All plates were analyzed using either a CTL reader (Immunospot, Cleveland, OH, USA) or an AID reader (AID Diagnostika GmbH, Strassberg, Germany). Since the vaccine induced antigen-specific B-cell responses were expected to vary at the selected time points, different concentrations of PBMC were added to the wells in the ELISpot plate. The cell concentrations selected had been evaluated earlier (data not shown) and the concentrations were as follows; days 0 and 28–42: 2 × 105 PBMC/well, days 7 and 14: 1 × 105 PBMC/well, and month 3: 4 × 105 PBMC/well. All cells were added in a two-fold serial
titration; the wells with the lowest concentration were only used if the highest concentration yielded a too numerous amount of spots to count. As a control for non-specific spots, unstimulated as well as stimulated cells were added in duplicates to blanco wells. Total IgG wells were used as a positive control 17-AAG nmr for each subject at each time point; if a sample generated low total IgG responses, the
sample was retested. Plasma blasts were defined as ASC detected in the wells of unstimulated cells after subtracting spots detected in the unstimulated blanco wells. Memory B cells were defined as the number of ASC in the wells with stimulated ADP ribosylation factor cells after the subtraction of plasma blasts and spots detected in the stimulated blanco wells. Antigen-specific plasma cell as well as memory B cell ASC was adjusted to ASC/1 × 106 PBMC for statistical analysis and should be considered as a relative number and not an absolute number of antigen-specific B cells. The Wilcoxon matched-pair signed rank test was used for the comparison between time points. All the data were considered non-parametric and p-values < 0.05 were considered statistically significant. Statistical analyses were performed using GraphPad Prism (GraphPad Software Inc., San Diego, CA, USA). Ethical approval was obtained from the Regional Ethical Board in Stockholm (protocol 2009/1:1). A human IgG B-cell ELISpot assay based on new capture and detection mAbs was evaluated. Pinna et al. had previously established the R848 + IL-2 combination as the optimal B-cell activator (Pinna et al.
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