Figure 3
Figure 3. Expression of AML1-ETO, MPO, and clonality in leukemic cells. (A) Western blot analysis of 2 independent mice spleen cell samples and one bone marrow cell sample showing the expression of AML1-ETO. Kasumi cells serve as a positive control. (B) Bone marrow and spleen cells from recipient mice of p21Waf1-deficient cells expressing AML1-ETO and a control mouse were cytospun and stained for MPO and counterstained with Wright-Giemsa for the analysis of immature blasts. The arrows indicate MPO+ immature blasts in the leukemic mice and in the control sample MPO+ neutrophils in the bone marrow. Image acquisition was performed as described for Figure 2, using a 100×/1.30 oil-immersion objective lens. (C) gDNA was isolated from 3 leukemic p21Waf1−/− mice expressing AML1-ETO. The DNA was digested with BamHI and a Southern blot prepared. The blot was hybridized with the ETO probe 5′ of the BamHI site in ETO, washed, and exposed to film. The black dots indicate the integration signals.

Expression of AML1-ETO, MPO, and clonality in leukemic cells. (A) Western blot analysis of 2 independent mice spleen cell samples and one bone marrow cell sample showing the expression of AML1-ETO. Kasumi cells serve as a positive control. (B) Bone marrow and spleen cells from recipient mice of p21Waf1-deficient cells expressing AML1-ETO and a control mouse were cytospun and stained for MPO and counterstained with Wright-Giemsa for the analysis of immature blasts. The arrows indicate MPO+ immature blasts in the leukemic mice and in the control sample MPO+ neutrophils in the bone marrow. Image acquisition was performed as described for Figure 2, using a 100×/1.30 oil-immersion objective lens. (C) gDNA was isolated from 3 leukemic p21Waf1−/− mice expressing AML1-ETO. The DNA was digested with BamHI and a Southern blot prepared. The blot was hybridized with the ETO probe 5′ of the BamHI site in ETO, washed, and exposed to film. The black dots indicate the integration signals.

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