1 mouse macrophage cells by using soluble rPnxIIIA. With increasing rPnxIIIA concentrations, the cytotoxicity as determined from the amount of lactose dehydrogenase (LDH) released by the cells was increased during a 24-h incubation (Additional file 2). In addition, we examined and compared the cytotoxicity of 3 recombinant RTX proteins identified in P. pneumotropica toward J774A.1 cells. During a 4-h incubation, native rPnxIA, rPnxIIA, and rPnxIIIA Vistusertib cost exhibited
55.2% ± 7.2%, 45.2% ± 3.1% and 29.8% ± 7.1% cytotoxic to J774A.1 cells, respectively. Compared with previously found RTX proteins, rPnxIIIA was significantly Ricolinostat mouse less cytotoxic than rPnxIA and rPnxIIA (P < 0.05). Several RTX toxins have been recognized in a species-specific manner, and are found to be cytotoxic to leukocyte function-associated antigen-1 (LFA-1)-bearing LB-100 clinical trial cells [30–32]. To characterize the cytotoxicity of PnxIIIA toward J774A.1 mouse macrophage cells, it is important to assess the effect of the presence of the LFA-1 receptor in macrophage cells. Furthermore, we employed comparative analysis of PnxIIIA cytotoxicity by using parent J774A.1 cells and anti-CD11a
monoclonal antibody (MAb)-treated J774A.1 cells as a neutralizing antibody. Figure 2 shows the changes in cytotoxicity of both J774A.1 cells and anti-CD11a MAb-treated cells cultured with 1.0 μg/ml rPnxIIIA. During a 24-h incubation, approximately 20-50% of cytolysis was inhibited by the addition of anti-CD11a MAb. These results indicate that the presence of the LFA-1 receptor may be required for rPnxIIIA cytotoxicity toward J774A.1 cells. Figure 2 Changes in the cytotoxicity of the rPnxIIIA toward J774A.1 mouse macrophage cells. The cytotoxicity Tau-protein kinase was determined by the release of LDH from J774A.1 cells with or without treatment with anti-CD11a monoclonal antibody cultured with rPnxIIIA. ECM-binding ability and hemagglutination Figures 3A to 3D show the changes in absorbance at 620 nm (A620) when rPnxIIIA was gradually added to the ECM-coated 96-well plate; the changes in absorbance were determined by an enzyme-linked
immunosorbent assay (ELISA). rPnxIIIA adhered to all tested rodent ECMs, with adhesion increasing as the rPnxIIIA concentration increased. In particular, the A620 of collagen type I (Figure 3A) was highest among the tested rodent ECMs, followed by that of collagen type II (Figure 3B), which was the second most adhesive ECM at a concentration of 50 μg/ml. Although the A620 values of collagen type IV and laminin were lower than those of collagen type I and type II, rPnxIIIA was confirmed to bind to both ECMs at higher concentrations (Figure 3C and 3D). These results indicate that rPnxIIIA can bind to rodent ECMs. Figure 3 The binding ability and hemagglutination activity of the rPnxIIIA. The binding ability of rPnxIIIA to the ECMs as determined by ELISA (A to D) and hemagglutination activity of the rPnxIIIA with sheep erythrocytes (E).