Human B cells infected by Epstein-Barr virus (EBV) are activated and transformed to continuously proliferative lymphoblastoid cell line (LCL). The other B cell mitogens or antigens, however, only activate B cell activation for a limited time. Through the previous cDNA microarray analysis of our lab, the expression of various CD markers, cellular kinases and interferon-stimulated genes (ISGs) are altered significantly in human CD19+ B cells 3 days post EBV infection and in LCLs. To investigate the differences of CD markers expression profile among EBV infected B cells and the other mitogen activated B cells, the expression of the CD markers in EBV, CD40+IL-4, poly I:C and LPS infected/activated B cells are analyzed by flow cytometry. The B cell activation marker CD80 is up-regulated in all activated cells and the other CD markers are expressed in distinct level in different treatments. In addition, the mRNA expression of the cellular kinases and ISGs in EBV, CD40+IL-4, poly I:C, LPS and SpA infected/activated B cells are determined by RT-Q-PCR. Expression of a good proportion of cellular kinases and ISGs are modulated only in EBV infected B cells. In order to further dissect the regulation of ISGs by EBV, we demonstrate that transient expression of EBV latent membrane protein 1 (LMP1) in Akata EBV (-) cells significantly induced ISGs expression. Furthermore, the LMP1 C-terminal activating region 2 (CTAR2) domain is essential for ISGs induction and NF-