Dengue virus (DEN), the human pathogen leading to dengue fever (DF), is epidemic in tropical and subtropical areas around the world. The DEN envelope protein (E), the primary viral protein inducing protective immunity, is critical for membrane fusion and mediates binding to cellular receptors. The ectodomain of the E monomer could further be divided into three domains assigned to domain I, domain II and domain III (EDI, EDII, and EDIII) (Modis et al., 2003). According to previous and our laboratory’s epitope mapping studies, many type-specific neutralizing antibodies against individual flaviviruses were localized to EDIII and alteration of specific residues in EDIII contributed to the loss of binding of neutralizing monoclonal antibodies (MAbs). Furthermore, subneutralizing MAbs that cross-react with other flaviviruses mainly bound to EDI-II. On the other hand, the presence of subneutralizing DEN cross-reactive serum antibodies in human hosts seems to cause an increase in the severity of secondary DEN infections via antibody-dependent enhancement (ADE). The roles of B-cell epitopes on the EDs in DEN pathogenesis, however, are still blurred. Accordingly, we screened a panel of MAbs from our laboratory to define the interaction between EDs and cross-reactive and neutralizing MAbs. Identification of neutralizing and pathologic epitopes will be useful for improving therapeutics to these diseases. In this study, we identified a number of cross-reactive and type-specific MAbs with their recognized EDs through ELISA, western blot analysis and quantitative real-time PCR (QRT-PCR). Additionally, we found that MAbs which recognized EDIII usually displayed strong neutralizing activity while MAbs which bound to EDI-II were likely to cause sub-/non-neutralizing or enhancing effects on DEN infections frequently.