Opposite responses of nuclear spermidine N 8 ‐acetyltransferase and histone acetyltransferase activities to regenerative stimuli in rat liver

Experiments performed in different models of hepatic regeneration at the time of maximal DNA synthesis, determined by thymidine kinase activity assay, demonstrated that spermidine N 8 ‐acetyltransferase activity increased 48 hr after CCl 4 administration (2‐fold), 72 hr after CCl 4 plus phenobarbital (3‐fold) and 24 hr after partial hepatectomy (4.5‐fold). On the contrary, at these times histone acetyltransferase activity diminished (approximately twofold) and was unchanged compared with control values in the liver of hepatotoxin‐treated and hepatectomized rats, respectively. Histone acetylation was, however, enhanced 1.5‐fold before the onset of DNA replication (14 hr), and 3.4‐fold after the peak of DNA synthesis (32 hr) in the liver of hepatectomized rats. α‐Difluoromethylornithine, a specific and irreversible inhibitor of ornithine decarboxylase that was administered to hepatectomized rats, blocked polyamine synthesis, thymidine kinase activity and consequently liver regeneration 24 hr after the surgery. In those conditions, spermidine N 8 ‐acetyltransferase activity was decreased approximately twofold, whereas histone acetyltransferase activity was elevated approximately twofold. All these effects were reversed by putrescine coadministration. Altogether, these findings showed that nuclear spermidine N 8 ‐acetyltransferase and histone acetyltransferase activities were regulated in opposite ways during the processes associated with liver regeneration. Moreover, they suggested that the polyamines themselves might have a direct or indirect role in this regulation. (H EPATOLOGY 1992;15:928–933).