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Vol. 53, Issue 3, 475-482, March 1998
Department of Medical Nutrition, Karolinska Institute, NOVUM, S-141
86 Huddinge, Sweden (H.H., M.M., M.P.-H., T.R., J.-A.G., M.W.),
Center
for Nutrition and Toxicology, NOVUM, Huddinge, Sweden (H.H., M.W.),
Department of Anatomy, Medical School, University of Tampere, Tampere,
Finland (M.P.-H.), and
Department of Pathology, Tampere University
Hospital, Tampere, Finland (M.P.-H.)
On isolation of rat breast cytochrome P450, one of the proteins whose
amino terminus was sequenced was CYP2A3. CYP2A3 was detected by Western
blotting in cytochrome P450 fractions isolated from breast of 3-, 6-, and 9-week-old rats but was low during pregnancy and lactation. Reverse
transcription-polymerase chain reaction analysis and sequencing of the
PCR product confirmed the presence and identity of CYP2A3 in the rat
breast. Breast microsomal coumarin-7-hydroxylase activity paralleled
the developmental pattern observed for CYP2A3 on Western blots. In the
lung, coumarin-7-hydroxylase activity was 10-fold higher than that in
the breast, but the developmental pattern was similar to that in the
breast. Lung microsomes from 9-week-old rats activated the heterocyclic
amine 2-amino-3-methylimidazo[4,5-f]quinoline to
mutagenic metabolites which could be detected with the Ames test. This
activation could be inhibited by the CYP2A3 antiserum. With breast
microsomes, which contain 
10% of the cytochrome P450 in the lung,
activation of 2-amino-3-methylimidazo[4,5-f]quinoline could not be reliably measured. Immunohistochemical localization revealed that CYP2A3 was expressed in a limited number of epithelial cells in the ducts of 6-week-old rat breast. Double staining with smooth muscle actin, a marker for myoepithelial cells, showed no
staining of CYP2A3 immunoreactive cells, indicating that these cells
were not myoepithelial. The data clearly show that a cytochrome P450
that can activate environmental procarcinogens is developmentally regulated and concentrated in specific cells in the breast. The peripubertal period seems to be a window in time when the breast may be
more sensitive to procarcinogens that are substrates for CYP2A3.
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