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Fig. 3. Cut and cell cycle regulation. ct mutant cells are marked by the
absence of histone-GFP (hGFP; green in A,B,D,E and white in
A'',D''). DAPI is shown in blue (A,B,B',E,e).
(A,A',A'') No Cut expression (shown in red in A and white in
A') was detected in ctdb7 mutant follicle-cell
clones (arrow). The sister clones (outlined and marked by higher levels of
GFP) had higher levels of Cut expression than the heterozygous
ctdb7 follicle cells. (B,B',B'')
ctdb7 mutant follicle cells had larger nuclei and less
CycA expression. In a stage 6 egg chamber, DAPI staining showed that
ctdb7 mutant follicle cells (outlined) had larger nuclei
than the wild-type cells. In the clone, CycA expression is absent (red in B
and B''), but in the neighboring wild-type cells about half of the cells
were CycA positive. (C) Number of nuclei in ctdb7 mutant
clones (blue bars) compared with that in their associated sister clones
(purple bars) in stage 10 egg chambers. The x-axis represents the clone
number, and the y-axis represents the number of cells per clone or
corresponding sister clone. (C') On average, the number of nuclei in the
clonal area was one third of that in the associated sister clone.
(D,D',D'') CycE (red in D and white in D') had normal
oscillating expression pattern in the clone cells (outlined). (E,E')
ctdb7 mutant follicle cells properly switched to the
gene-amplification stage. A foci-like pattern of BrdU incorporation (red in E
and white in E') was found in the cut-mutant follicle cells in
a stage 10B egg chamber. (e,e') The circled areas in E and E' show
four dots of BrdU incorporation foci (red in e and white in e') in each
nucleus.
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