Figure 2.
Figure 2. FACS analysis of leukemic mononuclear cells infiltrating the liver of founder mouse no. 13, comparison of hematologic parameters of transgenic progeny of no. 22, and molecular certification of p230 Bcr/Abl expression. (A) Surface marker analysis of leukemic cells infiltrating the liver of founder no. 13. (B) Comparison of hematologic parameters in the transgenic mice (n = 20; Tg, •) and nontransgenic controls (n = 10; C, ○) from 5 months to 15 months. The data are shown as the mean values and standard deviations for each group. Time course of WBC count, platelet (Plt) count, the percentage (%) of granulocytes, and hemoglobin (Hb) are shown. **P < .01; ***P < .001. (C) Northern blot analysis of p230 Bcr/Abl mRNA in tissues from no. 13 and no. 22 offspring. Lane K562: K562 cells as positive control; lane 32D: mouse 32D cells as negative control; lane liver no. 13: liver cells of no. 13; lane spleen no. 22: spleen cells of no. 22; lane spleen no. 13: spleen cells of no. 13; lane bone marrow no. 22: bone marrow cells of no. 22. The bottom bar shows the bands of glyceraldehyde-3-phosphate dehydrogenase (GAPDH) mRNA as an internal control. (D) P230 Bcr/Abl transgene product and (E) kinase activity of the p230 Bcr/Abl transgene product of the splenic cells. The expressed and phosphorylated P230 Bcr/Abl transgene products are indicated by arrows, and the positions of protein markers are shown on the right. The splenic cells of a 3-month-old F1 transgenic mouse were subjected to Western blot and immunoprecipitation analyses.

FACS analysis of leukemic mononuclear cells infiltrating the liver of founder mouse no. 13, comparison of hematologic parameters of transgenic progeny of no. 22, and molecular certification of p230 Bcr/Abl expression. (A) Surface marker analysis of leukemic cells infiltrating the liver of founder no. 13. (B) Comparison of hematologic parameters in the transgenic mice (n = 20; Tg, •) and nontransgenic controls (n = 10; C, ○) from 5 months to 15 months. The data are shown as the mean values and standard deviations for each group. Time course of WBC count, platelet (Plt) count, the percentage (%) of granulocytes, and hemoglobin (Hb) are shown. **P < .01; ***P < .001. (C) Northern blot analysis of p230 Bcr/Abl mRNA in tissues from no. 13 and no. 22 offspring. Lane K562: K562 cells as positive control; lane 32D: mouse 32D cells as negative control; lane liver no. 13: liver cells of no. 13; lane spleen no. 22: spleen cells of no. 22; lane spleen no. 13: spleen cells of no. 13; lane bone marrow no. 22: bone marrow cells of no. 22. The bottom bar shows the bands of glyceraldehyde-3-phosphate dehydrogenase (GAPDH) mRNA as an internal control. (D) P230 Bcr/Abl transgene product and (E) kinase activity of the p230 Bcr/Abl transgene product of the splenic cells. The expressed and phosphorylated P230 Bcr/Abl transgene products are indicated by arrows, and the positions of protein markers are shown on the right. The splenic cells of a 3-month-old F1 transgenic mouse were subjected to Western blot and immunoprecipitation analyses.

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