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Fig. 3. Changes in gene and protein expression following loss of IKK2.
(A) Western blot analysis for total and serine phosphorylated levels of
AKT, FOXO3a and of STAT3 at 24 hours' involution in mammary glands from
Cre-, Cre+/Ikk2fl/wt or
Cre+/Ikk2fl/fl mice. Significantly
increased levels of pAKT and pFOXO3a were seen in the absence of IKK2. Loading
control was 
-tubulin. (B) DAB immunohistochemistry for FOXO3a in
mammary gland sections from Cre-,
Cre+/Ikk2fl/wt or
Cre+/Ikk2fl/fl mice at 24 hours'
involution. Reduced nuclear FOXO3a staining was seen in
Cre+/Ikk2fl/fl glands (<).
Percentage of positively staining nuclei is indicated in the lower right
corner of each image. (C) A representation of previously obtained
microarray data showing expression of DR ligands throughout lactation and
early involution (Clarkson et al.,
2004). (D) qRT-PCR for the DR ligands: FASL, TNF, TRAIL and
TWEAK and DR TNFR1. Significant reductions in TWEAK (**
t<0.01), TNF (* t<0.05) and TNFR1 as
determined by the paired t-test, were seen in glands from
Cre+/Ikk2fl/fl mice compared with
Cre- control mice. Levels are arbitrary units and have been
normalised to cyclophilin A. (E) qRT-PCR for TWEAK of control and
15dPGJ2 treated undifferentiated KIM2 cells. Statistically
significant decreases in TWEAK mRNA as determined by the paired
t-test, were seen following 4 hours (**t<0.01)
and 8 hours (***t<0.005) of 15dPGJ2
treatment. Levels are arbitrary units and have been normalised to cyclophilin
A. Scale bar: 100 µm.
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