Abstract:The aim of this research was to develop an enzyme linked immunosorbent assay to detect zearalenone in grain samples.Three hybridoma cells named 2E8，2C7，6E11 were obtained after cell fusion and filtering by immunizing Balb/c mouses with conjugate of ZEN and keyhole limpet hemocyanin.The subtypes of three monoclonal antibody were identified with IgG1 for heavy chain and Kappa for light chain.The cell 2E8 was chosen for subsequent experiments.An indirect-competitive Enzyme-Linked Immunosorbent Assay（ELISA）was developed for the detection of zearalenone with high specificity and affinity after optimizing.The half maximal inhibitory concentration（IC50）was（0.13±0.02）ng/mL，the limit of detection（IC15）was（0.02±0.01）ng/mL while the the limits of detection are 2.4 μg/kg，4.0 μg/kg for corn and oat with the recoveries from 82.80%to 109.20%and the coefficients of variation was between 3.27%and 15.38%.The method was confirmed by high performance liquid chromatography tandem mass spectrometry with a good correlation.