Fig. 7. Aneuploidy, polyploidy and variable nuclear morphology in mutant Dm myb abdominal epidermal cells. (A,B) Abdominal epidermal samples from female pupae hybridized with an X-chromosome probe (red), and stained with DAPI (blue) and PH3 antibodies (green). (A) Two signals were seen in each of two separating nuclei in w/Df(1)sd^72a controls during anaphase. (B) By contrast, a different number of signals (1, 4 and 6) were evident in each of three separating nuclei in a mutant myb² cell. (C-K) Abdominal epidermal samples from females at 30 hours APF for controls and at 44-46 hours APF for Dm myb mutants were stained with DAPI for DNA quantitation (blue in D-K) and rhodamine-labeled phalloidin (red in D-K), and optically sectioned by confocal microscopy under identical conditions. For each of three experiments, nuclear fluorescent intensities were measured. The average value of the G₁ control nuclei was determined and used as the base value of 1x. Values of other nuclei were adjusted accordingly to calculate relative fluorescent intensities. (C) Results of analyzing 121 control (w/Df(1)sd^72a); 124 myb², and 83 myb²/Df(1)sd^72a nuclei are graphically represented. The range of values included in each category are indicated in parentheses as follows: 0.5x ( 0.6); 1x (0.7-1.5x); 2x (1.6-2.5x) and 3x ( 2.6). (D-K) Examples of control and mutant cells with relative DNA quantitation values as indicated. (D) Three control w/Df(1)sd^72a G₁ nuclei; (E) a control G₂ nucleus is centered; (F) enlarged myb² nucleus; (G) binucleate myb² cell; (H) mis-shapen and enlarged myb²/Df(1)sd^72a nucleus; (I) multilobed myb²/Df(1)sd^72a nucleus; (J) a myb²/Df(1)sd^72a nucleus with subdiploid DNA content (arrow); (K) a myb²/Df(1)sd^72a cell containing a large nucleus and a micronucleus indicated by arrow. Scale bars: in A, 0.01 mm in A,B; in K, 0.01 mm in D-K.