![Figure 5. Dual inhibition of MYD88 and Sp1 activity leads to synergistic killing in WM cells, and suppression of NF-κB activity. (A) BCWM.1 cells were transfected with either Scr or MYD88-specific siRNA; 24 hours after transfection, BCWM1 cells were treated with either vehicle or TMP and cultured for an additional 24 hours. Cell proliferation was assessed by thymidine uptake and presented as a percentage of control. (B) BCWM.1 cells were transfected with either Scr or MYD88-specific siRNA; 48 hours after transfection, WM cells were treated with either vehicle or TMP and cultured for an additional 4 hours. TNF-α was added for the last 20 minutes. NF-κB p65 TF binding to its consensus sequence on the plate-bound oligonucleotide was analyzed in nuclear extracts. The results represent means ± SD of triplicate experiments. (C-D) BCWM1 and MWCL1 cells were cultured in the absence or presence of IRAK 1/4 inhibitor peptide 407601 and TMP for 24 hours. Cell growth was assessed by [3H]thymidine uptake assay and presented as a percentage of control cells (untreated cells). Data are mean ± SD (n = 3). CIs and fractions affected were generated with CalcuSyn software for each set of combination. CI <1, CI values = 1, and CI values >1 indicate synergism, additive effect, and antagonism, respectively.](https://ash.silverchair-cdn.com/ash/content_public/journal/blood/123/17/10.1182_blood-2014-01-550509/4/2673f5.jpeg?Expires=1724170914&Signature=vIR9httdPk0OTlh39tUp4togVb9GveIme75mUpiek1df85D5Zz-bTBS6kZpX26nzETlPKHtVtuiukvrWSXs-OzsemeeG5lMkhQvp1KxngNSADBzWpqcqBIUxJ0bjHD~NAhliUchY01Tbm-5YqY3y1tu75ISDanXy4tikArMgWL06qcgcW1eXDOj5IjdoXfoq6gmN7nYc7llKIYtE1SZS798v-FLAklET7HlIkQf-31pvR1m2blJKyEZ7cq9p-tG8Utpx7J-Mh-9hRO0ZCbnDxSWV8U~-OJ7f7UlHZoosPfJ-B3mKzL-lFt0SHh01XyOdLAbxKo4uOnoXcjNI1k2hfg__&Key-Pair-Id=APKAIE5G5CRDK6RD3PGA)
Dual inhibition of MYD88 and Sp1 activity leads to synergistic killing in WM cells, and suppression of NF-κB activity. (A) BCWM.1 cells were transfected with either Scr or MYD88-specific siRNA; 24 hours after transfection, BCWM1 cells were treated with either vehicle or TMP and cultured for an additional 24 hours. Cell proliferation was assessed by thymidine uptake and presented as a percentage of control. (B) BCWM.1 cells were transfected with either Scr or MYD88-specific siRNA; 48 hours after transfection, WM cells were treated with either vehicle or TMP and cultured for an additional 4 hours. TNF-α was added for the last 20 minutes. NF-κB p65 TF binding to its consensus sequence on the plate-bound oligonucleotide was analyzed in nuclear extracts. The results represent means ± SD of triplicate experiments. (C-D) BCWM1 and MWCL1 cells were cultured in the absence or presence of IRAK 1/4 inhibitor peptide 407601 and TMP for 24 hours. Cell growth was assessed by [3H]thymidine uptake assay and presented as a percentage of control cells (untreated cells). Data are mean ± SD (n = 3). CIs and fractions affected were generated with CalcuSyn software for each set of combination. CI <1, CI values = 1, and CI values >1 indicate synergism, additive effect, and antagonism, respectively.
