![Figure 4. RAS and BCL-2 status of AML mice. (A) Percentage of peripheral blood BCL-2–positive cells in 4-week-old single transgenic (n = 10), untreated at 4-weeks old (day 0, n = 11), and posttreatment mice (postday 33, n = 14) showing a significant increase in BCL-2–positive cells with disease progression and after treatment (P < .0001). (B) Representative spleen cells from WT FVB/N, single and double MRP8[NRASD12/hBCL-2] AML transgenic mice assessed for total RAS and total BCL-2 expression by western blot analysis. Active RAS-GTP levels were measured via a sensitive RAF1-RBD pull down assay followed by western blot analysis with an anti-RAS antibody. Blots were reprobed with anti β-actin antibody to assess protein loading (n = 3). (C) Double MRP8[NRASD12/hBCL-2] AML untreated (day 0) and treated (+ABT-737) mice assayed (postday 33). Mice were assessed, as in (B). Histograms of RAS-GTP and hBCL-2 normalized to actin show an increase of the hBCL-2:RAS-GTP complex. The relative values were presented as fold increase over control samples as indicated (error bar = SD; n = 3). (D) Western blot analysis showing threonine 56 and serine 70 phosphorylations of hBCL-2 of spleen cells from untreated (day 0) and treated (postday 33), with β-actin showing equal protein loading (n = 2 mice). (E) MMP measurements by DiOC2(3) show a reduction of dye uptake in ABT-737–treated WT and AML mice relative to untreated samples (minimum in each group, n = 3 mice). (F) Confocal microscopy of stained cells of BM showing subcellular localization of RAS:BCL-2 complex from the AML mice shifting from mitochondrial localization (Mito, stained with Tom20+ antibody) in untreated (−) mice to plasma membrane (PM) localization (wheat germ agglutinin (WGA) after treatment (+) on postday 33. Rows 1 and 2 show pretreatment BM samples with RAS and BCL-2 co-localizing with the mitochondria (pale), whereas the pink coloration with the WGA antibody is consistent with co-localizations of RAS and BCL-2 with virtually no plasma membrane staining; rows 3 and 4 are 2 independent mice posttreatment probed with either Tom 20 (rows 3a and 3b) or WGA (rows 4a and 4b) showing the RAS:BCL-2 complex localizing in the plasma membrane with a white color, whereas with the mitochondrial antibody, green patches are visible with pale pink coloration in row 3a consistent with RAS and BCL-2 co-localizing in the absence of mitochondrial staining (in each group, n = 2 mice).](https://ash.silverchair-cdn.com/ash/content_public/journal/blood/122/16/10.1182_blood-2012-07-445635/4/2864f4.jpeg?Expires=1722720796&Signature=ob464PbIqbhADZDrwxr3U7KLzFFzPk6k50y8Y3t1g6JQA-6GMNAHPcuQbtBW50IqT~uWxTQmq~pjupzCSgeEo9Vs4nChz6tbrJz3ZiDGqbXmgpoLZQ0EArNiz53mYteG7ekl1qwVIb9wvJp0xnaQP82THO6i7gFifDaz9r8Ot6AY8yLKfybXD4TzALV9Srdal6YFeLd0ydOte4FoTtRoKJfwhzvu2emHlOA4IylOSoiTOLRJuf0L~JxzHo4rbtX6Oeej-lg0bN2JclckEj8JHC6FkyF2B0jc4X0JftSntPLtAF4MRXhSp5Rf4kLtsHfh0oDYIV-87~37QoVn9eZVfA__&Key-Pair-Id=APKAIE5G5CRDK6RD3PGA)
RAS and BCL-2 status of AML mice. (A) Percentage of peripheral blood BCL-2–positive cells in 4-week-old single transgenic (n = 10), untreated at 4-weeks old (day 0, n = 11), and posttreatment mice (postday 33, n = 14) showing a significant increase in BCL-2–positive cells with disease progression and after treatment (P < .0001). (B) Representative spleen cells from WT FVB/N, single and double MRP8[NRASD12/hBCL-2] AML transgenic mice assessed for total RAS and total BCL-2 expression by western blot analysis. Active RAS-GTP levels were measured via a sensitive RAF1-RBD pull down assay followed by western blot analysis with an anti-RAS antibody. Blots were reprobed with anti β-actin antibody to assess protein loading (n = 3). (C) Double MRP8[NRASD12/hBCL-2] AML untreated (day 0) and treated (+ABT-737) mice assayed (postday 33). Mice were assessed, as in (B). Histograms of RAS-GTP and hBCL-2 normalized to actin show an increase of the hBCL-2:RAS-GTP complex. The relative values were presented as fold increase over control samples as indicated (error bar = SD; n = 3). (D) Western blot analysis showing threonine 56 and serine 70 phosphorylations of hBCL-2 of spleen cells from untreated (day 0) and treated (postday 33), with β-actin showing equal protein loading (n = 2 mice). (E) MMP measurements by DiOC2(3) show a reduction of dye uptake in ABT-737–treated WT and AML mice relative to untreated samples (minimum in each group, n = 3 mice). (F) Confocal microscopy of stained cells of BM showing subcellular localization of RAS:BCL-2 complex from the AML mice shifting from mitochondrial localization (Mito, stained with Tom20+ antibody) in untreated (−) mice to plasma membrane (PM) localization (wheat germ agglutinin (WGA) after treatment (+) on postday 33. Rows 1 and 2 show pretreatment BM samples with RAS and BCL-2 co-localizing with the mitochondria (pale), whereas the pink coloration with the WGA antibody is consistent with co-localizations of RAS and BCL-2 with virtually no plasma membrane staining; rows 3 and 4 are 2 independent mice posttreatment probed with either Tom 20 (rows 3a and 3b) or WGA (rows 4a and 4b) showing the RAS:BCL-2 complex localizing in the plasma membrane with a white color, whereas with the mitochondrial antibody, green patches are visible with pale pink coloration in row 3a consistent with RAS and BCL-2 co-localizing in the absence of mitochondrial staining (in each group, n = 2 mice).
