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Department of Medical Sciences, University of East Piedmont "Amedeo Avogadro," Novara, Italy
2To whom correspondence should be addressed.
We investigated whether changes in apoptosis and cell proliferation
induced by starvation and refeeding in rat liver may contribute to the
initiation mechanism of liver cancer by 20 mg/kg of diethylnitrosamine
(DENA). Rats were starved for 4 d, then refed and given 20 mg/kg
of DENA after 1 d of refeeding. Rat livers were examined before
and after DENA treatment to measure DNA loss and synthesis, the number
of the placental form of glutathione S-transferase (P-GST)
positive cells and their turnover. Four days of starvation depressed
cell replication, as indicated by the labeling index (LI), and induced
apoptosis, as shown by the decay of total DNA radioactivity and
apoptotic index (AI, TUNEL technique). After 1 d of refeeding, AI
significantly decreased and LI remained low, indicating that a high
percentage of S phase cells was not required for the DNA
damage due to 20 mg/kg of DENA. DENA induced apoptosis and the AI after
20 mg/kg of DENA was 3% in refed rats vs. 1% in fully-fed rats
5 d after DENA (P
0.05). Putative-initiated
P-GST-positive hepatocytes appeared after administration of 20 mg/kg in
refed rats, and they showed a higher LI (6%) than the surrounding
P-GST-negative cells 3 d after DENA (LI = 2%; P
0.01), while very few P-GST-positive cells were found in
fully-fed rats. These data indicate that starvation-induced
cell loss and the subsequent refeeding trigger cell proliferation that
gives a selective advantage to the cells initiated by 20 mg/kg of DENA
to grow in the livers of refed rats.
KEY WORDS: diethylnitrosamine rat liver apoptosis cell proliferation cancer
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