Figure 3.
Figure 3. Inhibition of BAX promoter activity by LMP-1 is mediated by the NF-κB pathway. (A) Western blot for LMP-1 (top) and CAT assay (bottom) of HEK 293-T cells cotransfected with pBAX-CAT and with pHEBo (□) or pLMP-1 (▪) and with pcDNA-3 (columns 1-6) or pIκBα(S32/36A) (columns 7-8) and grown in the presence of 5 μg/mL CAPE (columns 3-4) or 100 μg/mL SN50 (columns 5-6). (B) Detection of p65 and p50 protein expression by Western blot (top) and CAT assay (bottom) of HEK 293-T cells cotransfected with pBAX-CAT and the vector pCMV-T (lane 1) or pCMV-T-p65 and pCMV-T-p50 in gradually changing ratios but at constant total amount (0.3 μg) (lanes 2-8) or with an IRF-1 expression plasmid (lane 9). *Significantly different from vector control (P < .05). (C) CAT assay as in panel B with pBAX-CAT replaced by pHIV-1-LTR-CAT. (D) Western blot for p65 and p50 expression (top) and CAT assay (bottom) of HEK 293-T cells cotransfected with pBAX-CAT and with vector pCMV-T (▪), equal amounts of pCMV-T-p65 and pCMV-T-p50 (□), or pCMV-T-p50 alone (▨) and with pcDNA-3 (columns 1-6) or pIκBα(S32/36A) (columns 7-9) and grown in the absence (columns 1-3, 7-9) or presence (columns 4-6) of 5 μg/mL CAPE. (E) Western blot for p65 (top) and p50 (bottom) in HEK 293-T cells cotransfected with pBAX-CAT and pCMV-T (left), pCMV-T-p65 (middle), or pCMV-T-p50 (right) expression plasmids and control siRNA (ctr-si), p65-siRNA (p65-si), or p50-siRNA (p50-si). (F) CAT assay of HEK 293-T cotransfected with pBAX-CAT (left) or pSV2-CAT (right) together with pHEBo (□) or pLMP-1 (▪) and with ctr-si, p65-si, or p65-si and p50-si. (G) CAT assay of 1852.4 cells grown 6 days in the absence (□) or presence (▪) of 2 μg/mL tetracycline, then transfected with pBAX-CAT and grown 3 days in the absence (left) or presence of 100 μg/mL SN50 (middle) or 1 μM Bay11-7082 (right). (A-D,F-G) CAT activity in control-transfected cells (first bar in each panel) was set to 100%. All experiments were performed in triplicate, and the mean and standard deviations are shown.

Inhibition of BAX promoter activity by LMP-1 is mediated by the NF-κB pathway. (A) Western blot for LMP-1 (top) and CAT assay (bottom) of HEK 293-T cells cotransfected with pBAX-CAT and with pHEBo (□) or pLMP-1 (▪) and with pcDNA-3 (columns 1-6) or pIκBα(S32/36A) (columns 7-8) and grown in the presence of 5 μg/mL CAPE (columns 3-4) or 100 μg/mL SN50 (columns 5-6). (B) Detection of p65 and p50 protein expression by Western blot (top) and CAT assay (bottom) of HEK 293-T cells cotransfected with pBAX-CAT and the vector pCMV-T (lane 1) or pCMV-T-p65 and pCMV-T-p50 in gradually changing ratios but at constant total amount (0.3 μg) (lanes 2-8) or with an IRF-1 expression plasmid (lane 9). *Significantly different from vector control (P < .05). (C) CAT assay as in panel B with pBAX-CAT replaced by pHIV-1-LTR-CAT. (D) Western blot for p65 and p50 expression (top) and CAT assay (bottom) of HEK 293-T cells cotransfected with pBAX-CAT and with vector pCMV-T (▪), equal amounts of pCMV-T-p65 and pCMV-T-p50 (□), or pCMV-T-p50 alone (▨) and with pcDNA-3 (columns 1-6) or pIκBα(S32/36A) (columns 7-9) and grown in the absence (columns 1-3, 7-9) or presence (columns 4-6) of 5 μg/mL CAPE. (E) Western blot for p65 (top) and p50 (bottom) in HEK 293-T cells cotransfected with pBAX-CAT and pCMV-T (left), pCMV-T-p65 (middle), or pCMV-T-p50 (right) expression plasmids and control siRNA (ctr-si), p65-siRNA (p65-si), or p50-siRNA (p50-si). (F) CAT assay of HEK 293-T cotransfected with pBAX-CAT (left) or pSV2-CAT (right) together with pHEBo (□) or pLMP-1 (▪) and with ctr-si, p65-si, or p65-si and p50-si. (G) CAT assay of 1852.4 cells grown 6 days in the absence (□) or presence (▪) of 2 μg/mL tetracycline, then transfected with pBAX-CAT and grown 3 days in the absence (left) or presence of 100 μg/mL SN50 (middle) or 1 μM Bay11-7082 (right). (A-D,F-G) CAT activity in control-transfected cells (first bar in each panel) was set to 100%. All experiments were performed in triplicate, and the mean and standard deviations are shown.

Close Modal
This Feature Is Available To Subscribers Only

or Create an Account

Close Modal
Close Modal