Five similar booster injections

were made 21, 36, 51, 66

Five similar booster injections

were made 21, 36, 51, 66 and 76 days later. Blood samples were drawn 1 week after the last injection. As a control, rabbits were also immunized with liposomes not containing Ibrutinib synthetic peptides, prepared as described previously [9]. Falcon flexible microtitration plates (Becton Dickinson France S.A.) were coated overnight at 4 °C with 5 μg/ml mut-II or L. muta muta whole venom in 0.02 M NaHCO3 buffer, pH 9.6, as described previously [3]. Absorbance values were determined at 492 nm with a Titertek Multiscan spectrophotometer. Tests were done in triplicate and the values represent means of experiments. Standard deviations are represented by error bars. Results were evaluated by Student’s t-test using Sigma Plot 10.0. In all cases, differences were considered significant at P < 0.05.

Hemorrhagic activity was assayed using the Kondo method [25] and adapted by Sanchez et al. [36]. Aliquots of L. muta muta venom in 100 μl physiological saline, or saline alone, were injected into the dorsal shaved skin of the non-immunized rabbits. Twenty-four hours later, the rabbits selleck inhibitor were euthanized and the back skin was totally removed in order to photograph and measure the hemorrhagic lesions. One minimum hemorrhagic dose (MHD) was defined as the dose which causes a hemorrhagic lesion 10 mm in diameter. The MHD of L. muta venom used throughout this study was 20 μg. For the in vivo neutralization assays of the hemorrhagic activity of L. muta venom, the immunized and control rabbits were challenged with L. muta venom

30 days after the last immunization by intradermal injection of an amount equivalent to 1 MND/kg. In order to map the epitope recognized by the neutralizing monoclonal antibody LmmAbB2D4, membrane-bound peptides of 15 amino acids, spanning the entire sequence of mut-II, were for probed with LmmAbB2D4. Only background reactivity was observed at the highest concentration of the polyclonal antibody (10 μg/ml; Fig. 1B – lower panel). As a control for peptide quality, the 15-mer peptides (Fig. 1A – upper panel) were reactive when probed with a rabbit polyclonal antiserum produced against mut-II. The phage-display system of expression of randomly generated peptides can identify peptides mimicking discontinuous epitopes (mimotopes). To identify peptides that would bind to LmmAbB2D4, four different phage libraries were screened, two of which expressed linear peptides of either 15 (X15) or 30 amino acids (X30), whereas the other two displayed peptides including either one or two fixed cysteines and whose sizes were 17 (XCX15) or 12 amino acids (XCX8CX). A significant enrichment of phage binding to the target antibodies was obtained after three rounds of biopanning (data not shown). Of approximately one hundred phage clones randomly picked from the third round of selection, seventeen clones were selected. The DNA sequence and the deduced amino acid sequence were determined (Fig.

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