Figure 3
Figure 3. Deletion of Notch1 accelerates T-ALL development. (A) Survival curves of IkL/LNotch1f/fCD4-Cre+ (IN1C+), IkL/LNotch1f/fCD4-Cre− (IN1C−), and IkL/LNotch1+/+CD4-Cre+ (IC+) mice. The P value corresponds to the statistical difference between the survival of IN1C+ and IN1C− mice by log-rank test. (B) PCR analysis of the deletion of the floxed sequences in a panel of IN1C+ tumors. (C) Thymocyte CD4/CD8 profiles (top) and photos of the thoracic cavity (bottom) from 7-week-old WT, IN1C−, and IN1C+ mice. (D) Surface Notch1 and CD25 expression of IN1C+ and IN1C− tumor cells and WT thymocytes. The immunoglobulin G isotype control is shown in the left panels. Similar results were observed in all IkL/L/IN1C− and IN1C+ mice analyzed (n > 10). (E) Transcriptome profiling of Notch target genes in 3 IN1C+ and 3 IN1C− tumors using Affymetrix 430 2.0 arrays. The data were normalized with those from leukemic T cells of Tel-Jak2 tg mice24 and from WT DN3, DN4, and DP thymocytes using the Robust Microarray Analysis algorithm. Red and green colors indicate high and low expression, respectively. (F) Proliferation of IN1C+ and IN1C− cell lines in the absence or presence of γ-secretase inhibitor over 6 days. Representative of 3 independent experiments. (G) Western blot of ΙCN1 expression in IN1C+ tumors using the Val1744 antibody. β-actin was used as a loading control. T99 is a IRC+ tumor that expresses ICN1 proteins of the normal 120 kDa size. The asterisk in the right panel points to likely degradation products. (H) PEST region sequences of IN1C+ tumors. The bold nucleotides correspond to insertions in the WT sequence. ICN1 proteins from samples T34, T6, and T49 are shown in supplemental Figure 1C; T51, T70 and T110 are shown in Figure 3G; T1 and T2 correspond to IN1C+ cell lines described in supplemental Figure 2. Numbering according to the Notch1 reference sequence NM_008714.

Deletion of Notch1 accelerates T-ALL development. (A) Survival curves of IkL/LNotch1f/fCD4-Cre+ (IN1C+), IkL/LNotch1f/fCD4-Cre (IN1C), and IkL/LNotch1+/+CD4-Cre+ (IC+) mice. The P value corresponds to the statistical difference between the survival of IN1C+ and IN1C mice by log-rank test. (B) PCR analysis of the deletion of the floxed sequences in a panel of IN1C+ tumors. (C) Thymocyte CD4/CD8 profiles (top) and photos of the thoracic cavity (bottom) from 7-week-old WT, IN1C, and IN1C+ mice. (D) Surface Notch1 and CD25 expression of IN1C+ and IN1C tumor cells and WT thymocytes. The immunoglobulin G isotype control is shown in the left panels. Similar results were observed in all IkL/L/IN1C and IN1C+ mice analyzed (n > 10). (E) Transcriptome profiling of Notch target genes in 3 IN1C+ and 3 IN1C tumors using Affymetrix 430 2.0 arrays. The data were normalized with those from leukemic T cells of Tel-Jak2 tg mice24  and from WT DN3, DN4, and DP thymocytes using the Robust Microarray Analysis algorithm. Red and green colors indicate high and low expression, respectively. (F) Proliferation of IN1C+ and IN1C cell lines in the absence or presence of γ-secretase inhibitor over 6 days. Representative of 3 independent experiments. (G) Western blot of ΙCN1 expression in IN1C+ tumors using the Val1744 antibody. β-actin was used as a loading control. T99 is a IRC+ tumor that expresses ICN1 proteins of the normal 120 kDa size. The asterisk in the right panel points to likely degradation products. (H) PEST region sequences of IN1C+ tumors. The bold nucleotides correspond to insertions in the WT sequence. ICN1 proteins from samples T34, T6, and T49 are shown in supplemental Figure 1C; T51, T70 and T110 are shown in Figure 3G; T1 and T2 correspond to IN1C+ cell lines described in supplemental Figure 2. Numbering according to the Notch1 reference sequence NM_008714.

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