Figure 6.
Molecular characterization of SU5614-resistant cells. (A) The juxtamembrane region of FLT3 was amplified by PCR with the use of the published primer pair 11F and 12R,48,49 and PCR products were separated by agarose gel electrophoresis and viewed under UV illumination after ethidium bromide staining. M indicates DNA molecular weight marker; H2O, water control; Ba/F3, native Ba/F3 cells; WT, Ba/F3 FLT3-WT; ITD, Ba/F3 FLT3-ITD; ITD-R1-4, Ba/F3 FLT3-ITD-R1-4; PP, positive control (patient with AML carrying a FLT3-LM). (B) Detection of FLT3-TKD mutations was performed by melting curve analysis after amplification of a 244-bp fragment by real-time PCR as described previously.50 In the presence of the FLT3-TKD wild-type sequence or the FLT3 TKD mutant DNA the fluorescence peak is observed at 63°C and 55°C, respectively. (C) The structural domains of the FLT3 protein with the position of the TKD mutation found in Ba/F3 FLT3-ITD-R1-4 cells (D835N and Y842H) are shown.