Figure 2
Figure 2. Effect of KIT D816V on Lyn and Btk activation in HMC-1 cells and Ba/F3 cells. (A) HMC-1.1 and HMC-1.2 cells were kept in control medium or in the presence of 1μM midostaurin for 4 hours. Thereafter, Western blot (WB) analysis was performed using Abs directed against p-LynTyr507, p-SrcTyr416, Lyn, p-BtkTyr223, Btk, and KIT. Moreover, the phosphorylation of KIT was analyzed by immunoprecipitation using an anti-KIT Ab followed by immunoblotting using an anti-phosphotyrosine Ab. The β-actin control is also shown. To confirm the specificity of this WB result, we also performed immunoprecipitation experiments using anti-Lyn Ab followed by immunoblotting with anti-pSrcTyr416 and anti-pLynTyr507 as well as anti-phospho-Ab 4G10. Again, midostaurin failed to suppress expression of p-Lyn (not shown). (B) Ba/F3 cells with doxycycline-inducible expression of wt KIT (Ton.Kit.wt) or KIT D816V (Ton.Kit.D816V) were kept in control medium or in the presence of doxycycline (doxy, 1 μg/mL) for 24 hours. In case of Ton.Kit.wt, SCF (100 ng/mL) was added to induce KIT phosporylation for 15 minutes. Thereafter, cells were harvested and subjected to Western blot analysis using an anti-phosphotyrosine Ab for detection of activated KIT and Abs directed against p-LynTyr507, p-SrcTyr416, Lyn, p-BtkTyr223, Btk, and phosphorylated STAT5 (p-STAT5) as well as total STAT5. Ba/F3 cells stably expressing BCR/ABL T315I (Ba/F3p210T315I) served as a positive control. The dual bands observed with Abs against Lyn and STAT5 in Ton.Kit.D816V cells may be explained by alternative splicing.

Effect of KIT D816V on Lyn and Btk activation in HMC-1 cells and Ba/F3 cells. (A) HMC-1.1 and HMC-1.2 cells were kept in control medium or in the presence of 1μM midostaurin for 4 hours. Thereafter, Western blot (WB) analysis was performed using Abs directed against p-LynTyr507, p-SrcTyr416, Lyn, p-BtkTyr223, Btk, and KIT. Moreover, the phosphorylation of KIT was analyzed by immunoprecipitation using an anti-KIT Ab followed by immunoblotting using an anti-phosphotyrosine Ab. The β-actin control is also shown. To confirm the specificity of this WB result, we also performed immunoprecipitation experiments using anti-Lyn Ab followed by immunoblotting with anti-pSrcTyr416 and anti-pLynTyr507 as well as anti-phospho-Ab 4G10. Again, midostaurin failed to suppress expression of p-Lyn (not shown). (B) Ba/F3 cells with doxycycline-inducible expression of wt KIT (Ton.Kit.wt) or KIT D816V (Ton.Kit.D816V) were kept in control medium or in the presence of doxycycline (doxy, 1 μg/mL) for 24 hours. In case of Ton.Kit.wt, SCF (100 ng/mL) was added to induce KIT phosporylation for 15 minutes. Thereafter, cells were harvested and subjected to Western blot analysis using an anti-phosphotyrosine Ab for detection of activated KIT and Abs directed against p-LynTyr507, p-SrcTyr416, Lyn, p-BtkTyr223, Btk, and phosphorylated STAT5 (p-STAT5) as well as total STAT5. Ba/F3 cells stably expressing BCR/ABL T315I (Ba/F3p210T315I) served as a positive control. The dual bands observed with Abs against Lyn and STAT5 in Ton.Kit.D816V cells may be explained by alternative splicing.

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