Metabolism of the {beta}-oxidized intermediates of N-nitrosodi-n-propylamine: N-nitroso-{beta}-hydroxypropylpropylamine and N-nitroso-{beta}-oxopropylpropylamine

doi:10.1093/carcin/22.3.499

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Carcinogenesis, Vol. 22, No. 3, 499-506, March 2001
© 2001 Oxford University Press

CARCINOGENESIS

Metabolism of the ß-oxidized intermediates of N-nitrosodi-n-propylamine: N-nitroso-ß-hydroxypropylpropylamine and N-nitroso-ß-oxopropylpropylamine

John F. Teiber¹^,2, Katherine Macé³ and Paul F. Hollenberg²^,4

¹ Department of Environmental and Industrial Health and
² Department of Pharmacology, The University of Michigan, Ann Arbor, MI 48109-0632, USA and
³ Nestlé Research Center, PO Box 44, CH-1000, Lausanne 26, Switzerland

The rat liver carcinogen N-nitrosodi-n-propylamine (NDPA) ismetabolized to a propylating and methylating species in vivo.Metabolism to a methylating species is believed to require aninitial hydroxylation by cytochrome P450s (P450s) to N-nitroso-ß-hydroxypropylpropylamine(NHPPA), which is oxidized to N-nitroso-ß-oxopropylpropylamine(NOPPA), followed by a P450-mediated depropylation to ß-oxopropyldiazotate,which non-enzymatically breaks down to the methylating agent.Purified rat liver P450 2B1 and rabbit liver 2E1 in the reconstitutedsystem and liver microsomes from phenobarbital (PB) and pyridine(Pyr) treated rats readily metabolized NOPPA to a methylatingspecies as determined by the in vitro formation of 7-methylguanine(m⁷Gua) in DNA. Exposure of cells derived from the human liverepithelium transfected with human 2E1 (T5-2E1) to NOPPA resultedin the formation of m⁷Gua DNA adducts and a dose dependent toxicity.In vitro incubation of NHPPA with microsomes from PB, Pyr andnon-treated (NT) rats and a human microsomal sample also resultedin m⁷Gua formation. P450s 2B1 and 2E1 oxidized NHPPA to NOPPA,forming 16.5 ± 3.1 and 20.0 ± 4.4 pmol NOPPA/pmolP450 in 1 h, respectively. Rat liver cytosol, in the presenceof NAD⁺, oxidized NHPPA to NOPPA at a rate of 13.7 ±3.0 pmol/min/mg protein while microsomes from NT rats catalyzedthis reaction at 95.6 ± 16.5 pmol/min/mg protein. Cellsderived from hamster lung tissue (V79 control) and T5-neo cellsoxidized NHPPA to NOPPA. This oxidation was about 15 fold higherin T5-2E1 or V79 cells transfected with human 2E1 or rat 2B1,respectively. The results are consistent with the putative sequentialoxidation pathway and suggest that, at the concentrations tested,oxidation of NHPPA to NOPPA may be predominantly mediated bycytochrome P450s. In addition, it appears that rabbit, rat andhuman P450 2E1 can catalyze both oxidations.

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