Development of immunoassay techniques to detect microcystin in environmental samples

The contamination of drinking water by cyanobacterial toxins is a public health issue and a concern for water authorities throughout the world. Microcystin-LR (MCLR) is a hazardous cyclic heptapeptide cyanotoxin, which inhibits protein phosphatase PP1 and PP2A in hepatocytes. Microcystins are produced by several genera of cyanobacteria and presents more than 70 structural variations characterized in natural blooms. As haptens, microcystins are unable to invoke an immune response in animals. Consequently, the application of conjugation methods with an additional carrier protein, the KLH (Keyhole Limpet Hemocyanin) was necessary. The main objective of this study was to obtain monoclonal (in mice) and polyclonal (in rabbits) antibodies for reacting against MCLR. In what refers to monoclonal antibodies, 9 hybridomas (k29, k210, k317, k248, k284, k290, k2161, k2226, k2232) were obtained; however only 5 were stables (k29, k317, k248, k284, k2232). These were selected to be isotyped, expanded in ascitic fluid, purified by protein-A column chromatography and then, they were titrated. Out of these five antibody-secretor hybridomas, clone k317 was the best to recognize (more specific) the MCLR toxins. Antibodies in hybridoma cell culture supernatant and purified ascites fluid were identified by ELISA assay (Enzyme Linked Immunosorbent Assay) as prior standardized. Even when sensitizing ELISA plate with different antigens, as MCLR-cBSA, MCLR, MCLR, MCRR, MCYR and MCLA, clone 17 presented the best linearity against microcystin variants. Therefore, the obtained clone 17 (isotype IgG1) is a promising clone and shall be used for detecting MCLR in drinking water through the development of a competitive ELISA immunoassay kit. In what refers to the polyclonal antibody, MCLR-mcKLH was used as immunization antigen, while MCLR-cBSA was used as sensitizing antigen for the IgG titration assay by indirect ELISA. In the sequence, a competition ELISA assay was standardized using the MCLR toxin as sensitizing antigen. This Casein method was standardized, validated and compared to the commercial kit Abraxis®. The competition ELISA kit using polyclonal antibody, known as Casein method, was analyzed concerning its Quantification Inferior Limit, Specificity, Selectivity, methanol influence of the assay, Recuperation, Linearity, Precision, Accuracy and Robustness. This screening method reached excellent results if compared to the commercial kit Abraxis®, for being able to detect both the microcystins variants and the nodularins in aquatic environmental. The competition ELISA assay using anti-MCLR polyclonal antibody was submitted to the grant of a patent by USP Innovation Agency (INPI 018090046230). (AU)