Human N-acetylation of benzidine : Role of NAT1 and NAT2

Human N-acetylation of benzidine : Role of NAT1 and NAT2

These studies were designed to assess metabolism of benzidine and N-acetylbenzidine by N-acetyltransferase (NAT) NAT1 and NAT2. Metabolism was assessed using human recombinant NAT1 and NAT2 and human liver slices. For benzidine and N-acetylbenzidine, Km and Vmax values were higher for NAT1 than for...

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Veröffentlicht in:Cancer research (Chicago, Ill.) Ill.), 1996-09, Vol.56 (17), p.3941-3947
Hauptverfasser: ZENSER, T. V, LAKSHMI, V. M, RUSTAN, T. D, DOLL, M. A, DEITZ, A. C, DAVIS, B. B, HEIN, D. W
Format: Artikel
Sprache:eng
Schlagworte:
Acetylation
Arylamine N-Acetyltransferase - metabolism
Base Sequence
Benzidines - metabolism
Benzidines - pharmacokinetics
Biological and medical sciences
Carcinogenesis, carcinogens and anticarcinogens
Chemical agents
Female
Genotype
Humans
Isoenzymes - metabolism
Kinetics
Liver - anatomy & histology
Liver - enzymology
Liver - metabolism
Male
Medical sciences
Middle Aged
Molecular Sequence Data
Phenotype
Recombinant Proteins - metabolism
Tumors
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Zusammenfassung:These studies were designed to assess metabolism of benzidine and N-acetylbenzidine by N-acetyltransferase (NAT) NAT1 and NAT2. Metabolism was assessed using human recombinant NAT1 and NAT2 and human liver slices. For benzidine and N-acetylbenzidine, Km and Vmax values were higher for NAT1 than for NAT2. The clearance ratios (NAT1/NAT2) for benzidine and N-acetylbenzidine were 54 and 535, respectively, suggesting that N-acetylbenzidine is a preferred substrate for NAT1. The much higher NAT1 and NAT2 Km values for N-acetylbenzidine (1380 +/- 90 and 471 +/- 23 microM, respectively) compared to benzidine (254 +/- 38 and 33.3 +/- 1.5 microM, respectively) appear to favor benzidine metabolism over N-acetylbenzidine for low exposures. Determination of these kinetic parameters over a 20-fold range of acetyl-CoA concentrations demonstrated that NAT1 and NAT2 catalyzed N-acetylation of benzidine by a binary ping-pong mechanism. In vitro enzymatic data were correlated to intact liver tissue metabolism using human liver slices. Samples incubated with either [3H]benzidine or [3H]N-acetylbenzidine had a similar ratio of N-acetylated benzidines (N-acetylbenzidine + N',N'-diacetylbenzidine/ benzidine) and produced amounts of N-acetylbenzidine > benzidine > N,N'-diacetylbenzidine. With [3H]benzidine, p-aminobenzoic acid, a NAT1-specific substrate, increased the amount of benzidine and decreased the amount of N-acetylbenzidine produced, resulting in a decreased ratio of acetylated products. This is consistent with benzidine being a NAT1 substrate. N-Acetylation of benzidine or N-acetylbenzidine by human liver slices did not correlate with the NAT2 genotype. However, a higher average acetylation ratio was observed in human liver slices possessing the NAT1*10 compared to the NAT1*4 allele. Thus, a combination of human recombinant NAT and liver slice experiments has demonstrated that benzidine and N-acetylbenzidine are both preferred substrates for NAT1. These results also suggest that NAT1 may exhibit a polymorphic expression in human liver.
ISSN:0008-5472
1538-7445