Nonhistone Protein Changes during the Diethylnitrosamine-induced Carcinogenesis of Rat Liver

1981 
Diethylnitrosamine (DENA) was administered with drinking water (40 mg/liter) to male Wistar rats for 4, 6, 8, and 10 weeks. The protein:DNA ratio and the ultraviolet light spectral properties of liver chromatin were not modified by DENA treat ment. Nonhistone proteins were separated by sodium dodecyl sulfate:polyacrylamide electrophoresis on slab gels and ana lyzed by densitometry with a scanning microphotometer con nected on line to a computer. There were no qualitative changes in the pattern of nonhistone proteins during the treat ment with DENA. The quantitative changes statistically signifi cant at p < 0.005 were detected only in the 4th and 10th week, increases in fractions with molecular weights of 41,000 to 47,000 and 51,000 to 64,000 and decreases in fractions with molecular weights of 27,000 to 32,000 and 47,000 to 51,000 having been found. The proteinase activity of liver chromatin was assayed in incubation mixtures with 0.2 and 2 M NaCI and the measure ment of the cleavage products was performed with ninhydrin. Proteolytic activity was found only in 0.2 M NaCI and was higher in rats treated for 8 weeks with DENA than in controls. Autolysis of chromatin for 24 hr at 37° showed a severe breakdown of the nonhistone protein, being greater in the highmolecular-weight fractions than in the low-molecular-weight
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