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Genetic Polymorphism of Human CYP2E1 - Molecular Pharmacology


0026-895X/97/030370-07$3.00/0 Copyright © by The American Society for Pharmacology and Experimental Therapeutics All rights of reproduction in any form reserved. MOLECULAR PHARMACOLOGY, 51:370 –376 (1997).

Genetic Polymorphism of Human CYP2E1: Characterization of Two Variant Alleles YIN HU, MIKAEL OSCARSON, INGER JOHANSSON, QUN-YING YUE, MARJA-LIISA DAHL, MARCO TABONE, ` EMANUELE ALBANO, and MAGNUS INGELMAN-SUNDBERG SARINO ARINCO, Departments of Medical Biochemistry and Biophysics (Y.H., M.O., I.J., M.I.-S.) and Laboratory Sciences and Technology (Q.-Y.Y., M.-L.D.), Huddinge University Hospital, Karolinska Institutet, Stockholm, Sweden, Department of Medical Sciences, University of Torino, Novara, Italy (E.A.), and Department of Medicine, University of Turin, Turin, Italy (M.T., S.A.)

SUMMARY Ethanol-inducible CYP2E1 is an enzyme of major toxicological interest because it metabolizes several precarcinogens, drugs, and solvents to reactive metabolites. CYP2E1 has also been implicated in alcohol liver disease because of its contribution to oxidative stress. Previously, polymorphic alleles with mutations in introns and in the 59-flanking regulatory region have been described, and their presence has been related to the incidence of alcohol liver disease and lung cancer. In the present investigation, we investigated whether any functional mutations are linked to the above-mentioned rare alleles and also screened for mutations in the open reading frame using single-stranded conformation polymorphism and genomic DNA from almost 200 individuals belonging to either a Chinese, an Italian, or a Swedish population. Two new CYP2E1 gene variants were found with functional mutations: one (CYP2E1*2) in which a G1168A point mutation in exon 2 caused an R76H amino acid substitution, and the other (CYP2E1*3) in which a G10059A

Ethanol-inducible CYP2E1 has received much attention because of the potentially important toxicological roles of this enzyme. The enzyme is localized mainly in the liver but is also expressed and induced in the brain after ethanol treatment or ischemia (1, 2) and furthermore is distributed in many other tissues (3). The physiological role of this enzyme seems to be connected mainly with the conversion of acetone to gluconeogenetic precursors. Among the more than 70 different substrates specifically metabolized by this enzyme are most organic solvents, paracetamol, and several precarcinogens such as dimethylnitrosamine and ethanol (3, 4). In addition, CYP2E1 causes oxidative stress, and the oxy radicals generated by this enzyme are able to initiate NADPHdependent lipid peroxidation with the concomitant production of cytotoxic aldehydes. These have been implicated in ethanol-mediated hepatotoxicity (5). Thus, any functional This work was supported by grants from The Swedish Alcohol Research Fund and from The Swedish Medical Research Council.

base substitution in exon 8 yielded a V389I amino acid exchange. The corresponding CYP2E1 cDNAs were constructed, subcloned into the pCMV4 expression vector, and expressed in COS-1 cells. The cellular levels of CYP2E1 mRNA, CYP2E1 protein, and rate of chlorzoxazone hydroxylation were monitored. The CYP2E1*3 cDNA variant was indistinguishable from the wild-type cDNA on all variables investigated, whereas CYP2E1*2 cDNA, although yielding similar amounts of mRNA, only caused 37% of the protein expression and 36% of the catalytic activity compared with the wild-type cDNA. Complete screening by single-stranded conformation polymorphism of the three populations studied revealed that these variant alleles were rare. We conclude that the human CYP2E1 gene is functionally surprisingly well conserved compared with other cytochrome P450 enzymes active in drug metabolism, which suggests an important endogenous function in humans.

polymorphism of this enzyme might be an important factor in determining the relative risk of alcohol-mediated hepatotoxicity, any form of cancer, or susceptibility for drug toxicity. With respect to the metabolism of drugs used for clinical purposes, CYP2E1 can be considered to be among the six most important P450s, which also include CYP1A2, CYP2C9, CYP2C19, CYP2D6, and CYP3A4. Among the clinically important drug substrates for CYP2E1 are enflurane, halothane, isoniazid, chlorzoxazone, paracetamol, and theophylline (6). Because CYP2C9, CYP2C19, and CYP2D6 have been shown to exhibit functional polymorphisms (7), it might be assumed that similar inactivating mutations also would occur in the CYP2E1 gene and that their distribution might be of importance for the efficacy of drug treatment or for interindividual differences in toxicity exerted by paracetamol, for example. In line with this hypothesis, it has been demonstrated that there are important interindividual differences in the expression of human hepatic CYP2E1 (8, 9).

ABBREVIATIONS: P450, cytochrome P450; PCR, polymerase chain reaction; RFLP, restriction fragment length polymorphism; SSCP, singlestranded conformation polymorphism. 370

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Received July 15, 1996; Accepted December 5, 1996

Genetic Polymorphism of the Human CYP2E1 Gene

Materials and Methods Isolation of genomic DNA. Blood samples were obtained from healthy Swedish and Chinese control subjects and Italian alcoholic cirrhosis patients as described in previous publications (17–19). Genomic DNA was isolated using a guanidinium-isothiocyanate method or using the phenol extraction method (20). The studies were approved by the ethics committee at Karolinska Institutet. Construction of genomic libraries. The genomic libraries were made from subjects homozygous for the DraI C and DraI D alleles, respectively. When isolated, the DraI C allele exhibited mutations determined by RsaI and TaqI RFLP but was of the c1 genotype with respect to the 59-upstream polymorphic site at 21019 bp (21). Genomic DNA was partially digested by the restriction enzyme Sau3AI and ligated to a lEMBL3 vector. Positive plaques were identified by hybridization with 32P-labeled human CYP2E1 cDNA. SSCP analysis. One microliter of genomic DNA (;0.5 mg/ml) was amplified using the primers listed in Table 1. The PCR was carried out with initial denaturation for 1.5 min at 94°, followed by 35 cycles, each involving denaturation at 94° for 1 min, annealing at 52° for 1 min, and extension at 72° for 1 min. Five microliters of the PCR products was digested by an appropriate restriction enzyme in a total volume of 35 ml to yield 100- to 200-bp fragments. Subsequently, 15 ml of loading buffer containing 95% formamide, 20 mM EDTA, bromphenol blue, and xylene cyanol FF was added. Just before loading, the samples were heated to 95° for 5 min. Conformation polymorphisms of single-stranded DNA fragments were then analyzed using nondenaturing 8.7% polyacrylamide gels with 10% glycerol in a Hoeffer (San Francisco, CA) standard vertical SE 500slab gel unit. The gels were run in 23 Tris/borate/EDTA buffer (0.18 M Tris base, 0.18 M boric acid, and 0.004 M EDTA), at 4° for 4 hr at 270 V, and the DNA fragments were visualized by silver staining. DNA sequencing. DNA was amplified by PCR with primers, as shown in Table 1. One of the primers was biotinylated, and the PCR reaction was conducted as described above. Forty microliters of PCR products was mixed with Dynabeads M-280 Streptavidin (Dynal AS; Oslo, Norway), which was designed as a matrix for simple and efficient separations of biotinylated compounds. DNA strands were separated with 0.1 M NaOH using the Dynal Magnetic Particle Concentrator. Sequencing of DNA was carried out by the dideoxy

TABLE 1 Locations and sequences of primers used for PCR and DNA sequencing Primer


P1 P2 P3 P4 P5 P6 P7 P8 P9 P10 P11 P12 P13 P14 P15 P16 P17 P18 P19 P20 P21

22653–22636 276–261 288–305 1026–1043 1350–1367 4131– 4148 4433– 4450 4672– 4689 5024–5041 5257–5274 5572–5589 6333– 6350 6532– 6549 7516–7532 8034– 8051 9294–9311 9598–9615 9968–9985 10244–10261 10996–11013 11451–11468





b b

b b

b indicates that the primer is biotinylated.

chain-termination method using Sequenase version 2.0 T7 DNA polymerase (United States Biochemical, Cleveland, OH) and a-35Slabeled dATP (Amersham, Buckinghamshire, UK). Site-directed mutagenesis. Mutant CYP2E1 cDNAs containing the G1168A or G10059A (numbering based on genomic DNA) mutations were generated with the USE mutagenesis kit (Pharmacia Biotech, Uppsala, Sweden), using a human CYP2E1 wild-type cDNA subcloned into the pBluescript KS1 vector (Stratagene, La Jolla, CA), and mutagenic primers 59-GCTCGCAGCACATGGTGGT-39 and 59-GGCACAGTCATAGTGCCAA-39, respectively. The three cDNAs were subsequently subcloned into the pCMV4 expression vector (22) using the restriction sites HindIII and XbaI. Expression of mutated cDNAs. COS-1 cells were transfected with the pCMV4 constructs as previously described (18). After incubation for 72 hr, the cells were harvested in 100 mM sodium phosphate buffer, pH 7.4. Quantification of CYP2E1 mRNA and apoprotein levels. Total RNA was prepared from transfected cells using the TriPure Isolation Reagent (Boehringer Mannheim, Mannheim, Germany). Northern blot analysis was performed as previously described (23). Cells for Western blot and chlorzoxazone 6-hydroxylation analysis were sonicated for 20 3 1 sec and centrifuged at 10,000 3 g for 10 min at 4°. Supernatant corresponding to 10 mg of protein was subjected to sodium dodecyl sulfate gel electrophoresis using 8.7% polyacrylamide gels, and the proteins were subsequently transferred to a Hybond C nitrocellulose filter (Amersham) and incubated with antirat CYP2E1 serum (24) and with horseradish-peroxidase–linked protein A (BioRad, Hercules, CA). The enhanced chemiluminescense method (Amersham) was used to visualize the proteins, and quantification was carried out using a personal densitometer (Molecular Dynamics, Sunnyvale, CA). Chlorzoxazone 6-hydroxylation assay. Cell supernatant (10,000 3 g) corresponding to 300 mg of protein was incubated at 37° in 100 mM sodium phosphate buffer, pH 7.4, with 1 mM chlorzoxazone, 1 mM NADPH, and 28 pmol of rat P450 reductase [purified as described by Ingelman-Sundberg and Glaumann (25)] in a total volume of 500 ml for 180 min. The addition of reductase makes CYP2E1 the rate-determining factor, because the endogenous reductase levels in the COS cells are small. The reaction was terminated by the addition of 50 ml of 43% orto-phosphoric acid, and 1 mg of acetaminophen was added as an internal standard. Extraction of samples with dichloromethane and analysis of the amount of 6-OH-

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Analysis and characterization of polymorphisms in the CYP2E1 gene has hitherto involved mainly RFLP analysis using the restriction endonucleases DraI, TaqI, and RsaI. The polymorphic sites localized in introns and in the 59flanking region have been monitored in this way (10, 11). Molecular epidemiological studies have been carried out to relate the occurrence of these variant alleles, in particular, the DraI C allele, which has a mutation in intron 6 (allele frequency: Caucasians 10%, Asians 26%) and at 21019 bp (c1/c2) in the 59-upstream region [allele frequency: Caucasians 4%, Asians 20% (3)], to the incidence of lung cancer, susceptibility for alcohol liver disease (10 –14), inducibility of the enzyme by ethanol (15), and in vivo activity (15, 16). We evaluated whether these polymorphic sites are associated with any functional mutations in the open reading frame and, furthermore, examined to what extent the human CYP2E1 gene as such exhibits allelic variations in the open reading frame. For this purpose, we screened genomic DNA for mutations from two Caucasian and one Asian population using SSCP. The results indicate that the human CYP2E1 gene is highly conserved in these populations compared with other human P450 genes with products active in the metabolism of xenobiotics.



Hu et al.

chlorzoxazone formed was carried out with an high pressure liquid chromatography system using an electrochemical detector as described elsewhere (2). Linearity of the reaction for 180 min was established in all cases.

Results Two genomic libraries were constructed from two Caucasian subjects homozygous for the DraI C and DraI D haplotypes, respectively. The C allele of the c1 genotype with respect to the polymorphism at 21019 bp (26) was fully sequenced in its open reading frame and in parts of the 39and 59-flanking regions. Several mutations compared with the DraI D allele (27) were seen in the flanking regions (Fig. 1), among them an insertion (guanine) at position 213 in the promoter region adjacent to the TATA-box. Some mutations in the 39-flanking region were in putative motifs determining mRNA stability, such as polyadenylation signal (Fig. 1). Furthermore, many mutations were seen in areas sequenced in intron 6, as well as in the more remote 59-upstream flanking regions. However, no mutations were found in any of the exons. To investigate any polymorphic alleles with functional mutations, SSCP analysis was carried out on all exons and exon-intron junctions using the genomic DNA of 198 subjects: 78 Swedish control subjects, 78 Chinese control subjects, and 42 Italian patients suffering from alcohol-induced liver cirrhosis. The exons were amplified by PCR using the primers listed in Table 1, and the products were digested by appropriate restriction endonucleases to yield 100- to 200-bp fragments. In two of the 78 Chinese subjects, the SSCP analysis revealed a mobility difference of the PCR products from exon 2 obtained after digestion with RsaI (Fig. 2A). Direct sequencing revealed a G1168A point mutation (Fig. 2B), which caused an R76H amino acid substitution (Fig. 2C). The mutation is localized at a polymorphic restriction HhaI site (GCGC to GCAC) (Fig. 2C), and the allele was designated CYP2E1*2.1 1 A new nomenclature system has recently been proposed for CYP2D6 alleles (40). This system is based on general recommendations for allele no-

Using the same approach, we also found that 1 of the 42 Italian alcoholic cirrhosis patients showed a unique pattern in the SSCP analysis of exon 8 (Fig. 3A). Sequence analysis revealed a G10059A mutation (Fig. 3B), which caused a V389I amino acid substitution (Fig. 3C). This allele was designated CYP2E1*3.1 Using SSCP and sequence analysis, we identified a point mutation, G235T, only 2 bp downstream of the basal transcription element in the 59-flanking region (data not shown). To evaluate the functional importance of the mutations in the CYP2E1*2 and CYP2E1*3 alleles, site-directed mutagenesis was used to introduce these mutations into the wild-type CYP2E1 cDNA. The cDNAs were inserted into the pCMV4 expression vector and subsequently expressed in COS-1 cells. For comparison, cells transfected with the vector alone were used as negative controls. The amount of CYP2E1 mRNA was detected by Northern blot, and the CYP2E1 apoprotein levels were quantified by Western blot. The CYP2E1-dependent catalytic activities were determined by measuring NADPHdependent hydroxylation of chlorzoxazone in 10,000 3 g supernatants of the transfected cells. All constructs except the pCMV4 vector yielded CYP2E1 mRNA and immunodetectable CYP2E1 apoprotein. No major differences in mRNA levels were noticed in cells transfected with either of the three different cDNAs (Fig. 4, A and B). The level of CYP2E1 apoprotein in cells transfected with CYP2E1*2 cDNA was approximately 37% of that obtained in cells transfected with CYP2E1*1 cDNA (Fig. 4C). When 6-hydroxylation of chlorzoxazone was measured in the cell homogenates, a similar decrease was seen in activities as monitored on the protein level. By contrast, cells transfected with CYP2E1*3 cDNA had apoprotein levels and rates of chlorzoxazone 6-hydroxylation similar to that of cells transfected with CYP2E1*1 cDNA (Fig. 4D). The presence of these mutations in the populations invesmenclature, and the different alleles are denoted CYP2D6*n. Each allele is assigned a specific number. In accordance with this, we propose a similar system for designation of the CYP2E1 alleles with the following numbers: CYP2E1*1, wild-type sequence; CYP2E1*2, G1168A R76H; CYP2E1*3 G10059A V389I.

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Fig. 1. Schematic description of the results of sequence analysis of the DraI C allele of the human CYP2E1 gene. The areas sequenced were all exons and exon-intron junctions, bp 22788 to 22634, 21009 to 2809, 276 to 21, 7272 to 7892, and 11261 to 11710. DNA fragments of the exons amplified by PCR using the specific primers (P1–P21) and the location of amplified fragments are shown.

Genetic Polymorphism of the Human CYP2E1 Gene


Fig. 3. Identification of a functional mutation of exon 8 of the human CYP2E1 gene. A, SSCP analysis was performed using nondenaturing 8.7% polyacrylamide gels. Arrow (bottom), individuals who carry the mutation; arrow (side), extra bands seen in these samples. B, Direct PCR sequencing of exon 8 from wild-type and mutant individuals. Arrow, G10059A point mutation. C, Nucleotide sequence around the mutation in exon 8. Bold letter, point mutation for the codon V389I.

tigated was screened by SSCP. Two CYP2E1*2 alleles were found in the Chinese population and one CYP2E1*3 allele in the Italian population, whereas neither was present in the Swedish population studied (Table 2). This shows the high conservation of the open reading frame of the human CYP2E1 gene and indicates an important physiological function of this enzyme in vivo. No relationship between the distribution of these variant alleles and the previously described C/D and c1/c2 polymorphisms was found.

Discussion Much interest has been focused on the relationship between polymorphism of the human CYP2E1 gene as studied by RFLP and the incidence of lung cancer as well as the occurrence of alcoholic liver disease. In particular, two polymorphic loci, one in intron 6 (DraI C/D) and one in the 59-flanking upstream region (c1/c2) have received much attention. To evaluate any relationship between these polymor-

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Fig. 2. Identification of a functional mutation in exon 2 of the human CYP2E1 gene. A, The SSCP analysis was performed using nondenaturing 8.7% polyacrylamide gels. Arrow (bottom), individuals who carry the mutation; arrow (side), extra bands seen in these samples. B, Direct PCR sequencing of exon 2 from wild-type and mutant individuals. Arrow, G1168A point mutation. C, Nucleotide sequence around the mutation in exon 2. Bold letter, point mutation for the codon R76H; underlining, HhaI site.


Hu et al.

TABLE 2 Distribution of variant CYP2E1 alleles in the three different populations studied Base substitution Study population

G1168A (CYP2E1*2 )

G10059A (CYP2E1*3 )

No. of alleles

Chinese control subjects (n 5 78) Swedish control subjects (n 5 78) Italian cirrhosis patients (n 5 42)

2 0 0

0 0 1

phic alleles and any functional mutations and, furthermore, to investigate the occurrence of any mutations in the open reading frame, conditions for SSCP analysis were worked out to include all the exons and intron-exon junctions. Screening of a total of 198 individuals revealed that the coding part of the gene is well conserved among individuals and that only three alleles were found to cause amino acid exchanges. One of them, which had the R76H substitution (CYP2E1*2), caused less apoprotein levels and catalytic activity in the expression system, whereas no effect was seen on the mRNA level. The very similar decreases of both the protein and catalytic activity of this CYP2E1 variant suggests that the mutation does not affect the catalytic activity of the enzyme but that less protein is formed, perhaps because of a decreased translation efficiency or less stable protein. The expression system used does not, however, allow us to extrap-

olate this finding to the human in vivo situation. Our finding of a detrimental effect of the R76H substitution has to be confirmed in vivo using phenotype analysis with the chlorzoxazone of humans carrying the CYP2E1*2 allele in comparison to subjects homozygous for the CYP2E1*1 allele under otherwise identical conditions. The sensitivity for the detection of mutations by SSCP techniques using polyacrylamide gels in the absence or presence of glycerol has been found to be 90% and 70%, respectively (28). Some exons were run in the absence of glycerol, and additional bands were then obtained, but sequencing revealed no exon mutations.2 Statistically, we may have missed one additional mutation in one or two of the samples, although this would not change the conclusions drawn from the study. Because no crystal structure of CYP2E1 or any other mammalian P450 is available, alignments and homology-building models are used to make predictions concerning the localization of amino acids in the three-dimensional structure of the enzyme. None of the amino acid substitutions are located in the substrate recognition sites predicted by Gotoh (29) and are thus not expected to be directly involved in substrate binding. Hasemann et al. (30) made a structural alignment of three bacterial P450 structures and used this to align some of the mammalian P450 on the amino acid level. Using this 2

Y. Hu, unpublished observations.

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Fig. 4. Expression of wild-type and mutated CYP2E1 cDNAs in COS-1 cells. A and B, Northern blot analysis. CYP2E1 mNRA and b-actin mRNA were measured in cells transfected with the different mutants, and the ratio between CYP2E1 mRNA and b-actin mRNA levels were calculated. Twenty-five micrograms of total RNA was used for analysis. C, Western blot analysis of CYP2E1 showing densitometric quantification of CYP2E1 apoprotein levels in the cell homogenates. Levels are expressed as a percentage of the levels in the cells transfected with CYP2E1*1 cDNA. Inset, a representative Western blot from 10,000 3 g supernatant corresponding to 5 mg of protein per lane and rat liver microsomes as a control. LM, liver microsomes; NC, negative control, vector only. D, Catalytic activities. Chlorzoxazone 6-hydroxylation activity was measured in 10,000 3 g supernatants corresponding to 300 mg of protein. The reaction was linear with time for at least 180 min. The minute amount of 6-OH-chlorzoxazone formed in the cells transfected with the pCMV4 vector alone has been subtracted. The activity is expressed as a percentage of the activity seen in cells transfected with CYP2E1*1 cDNA. The results are data (mean 6 standard deviation) from four (B) or six (C and D) independent experiments performed in duplicate. Plasmids from at least two independent plasmid preparations were used for transfection.

Genetic Polymorphism of the Human CYP2E1 Gene

3 I. Dupont, D. Lucas, P. Clot, M. Seccia, C. Menez, and E. Albano, submitted for publication.

In conclusion, our data show that the open reading frame of the human CYP2E1 gene is surprisingly well conserved both in Asians and in Caucasians. This might suggest important endogenous functions and could indicate a pronounced endogenous role of this P450 in humans under certain conditions. Acknowledgments

Dr. Ylva Terelius, being homozygous for the DraI C allele, is gratefully acknowledged. References 1. Warner M., and J.-Å. Gustafsson. Effect of ethanol on cytochrome P450 in the rat brain. Proc. Natl. Acad. Sci. USA. 91:1019–1023 (1994). 2. Tindberg, N., H. A. Baldwin, A. J. Cross,and M. Ingelman-Sundberg. Induction of cytochrome P450 2E1 expression in rat and gerbil astrocytes by and inflammatory factors and ischemic injury. Mol. Pharmacol. 50: 1065–1072 (1996). 3. Ronis, M. J. J., K. O. Lindros, and M. Ingelman-Sundberg. The cytochrome P4502E subfamily, in Cytochromes P450, Pharmacological and Toxicological Aspects (I. Ioannides, ed.). CRC Press, Boca Raton, FL, 211–239. 4. Terelius, Y., K. O. Lindros, E. Albano, and M. Ingelman-Sundberg. Isozyme-specificity of cytochrome P450-mediated hepatotoxicity, in Frontiers Biotransformation (H. Rein and K. Ruckpaul, eds.). Vol. 8. Akademie Verlag, Berlin, 186–231 (1993). 5. Ingelman-Sundberg, M., I. Johansson, H. Yin, Y. Terelius, E. Eliasson, P. Clot, and E. Albano. Ethanol-inducible cytochrome P4502E1: genetic polymorphism, regulation, and possible role in the etiology of alcohol-induced liver disease. Alcohol 10:447–452 (1993). 6. Parkinson, A. An overview of current cytochrome P450 technology for assessing the safety and efficacy of new materials. Toxicol. Pathol. 24: 45–57 (1996). 7. Ingelman-Sundberg, M., and I. Johansson. The molecular genetics of the human drug metabolizing cytochrome P450s, in Advances in Drug Metabolism in Man (G. Pacifici and G. N. Fracchia, eds.). Office for Official Publications of the European Communities, Luxembourg, 543–586 (1995). 8. Ekstro¨m, G., C. von Bahr, and M. Ingelman-Sundberg. Human liver microsomal cytochrome P-450 IIE1. Immunological evaluation of its contribution to microsomal ethanol oxidation, carbon tetrachloride reduction and NADPH oxidase activity. Biochem. Pharmacol. 38:689–693 (1989). 9. Wrighton, S. A., P. E. Thomas, D. T. Molowa, M. Haniu, J. E. Shively, S. L. Maines, P. B. Watkins, G. Parker, G. Mendez-Picon, W. Levin, and P. S. Guzelian. Characterisation of ethanol-inducible human liver Nnitrosodimethylamine demethylase. Biochemistry 25:6732–6735 (1986). 10. Rannug, A., A. K. Alexandrie, I. Persson, and M. Ingelman-Sundberg. Genetic polymorphism of cytochromes P450 1A1, 2D6 and 2E1: regulation and toxicological significance. J. Occup. Environ. Med. 37:25–36 (1995). 11. Nedelcheva, V., I. Persson, I. Johansson, and M. Ingelman-Sundberg. Genetic polymorphism of human cytochrome P450 2E1. Methods Enzymol. 272:218–225 (1996). 12. Iwahashi, K. K., H. Nakamura, Y. Suwaki, Y. Matsuo, and Y. Ichikawa. Relationship between genetic polymorphism of CYP2E1 and ALDH2, and possible susceptibility to alcoholism. Alcohol Alcohol. 29:639–642 (1994). 13. Yu, M. W., A. Gladek-Yarborough, S. Chiamprasert, R. M. Santella, Y. F. Liaw, and C. J. Chen. Cytochrome P450 2E1, and glutathione Stransferase M1 polymorphisms and susceptibility to hepatocellular carcinoma. Gastroenterology 109:1266–1273 (1995). 14. Kato, S., M. Onda, N. Matsukura, A. Tokunaga, T. Tajiri, D. Y. Kim, H. Tsuruta, N. Matsuda, K. Yamashita, and P. G. Shields. Cytochrome P4502E1 (CYP2E1) genetic polymorphism in a case-control study of gastric cancer and liver disease. Pharmacogenetics 5:S141–S144 (1995). 15. Lucas, D., C. Menez, C. Girre, F. Berthou, P. Bodenez, I. Joannet, E. Hispard, L.-G. Bardou, and J.-F. Menez. Cytochrome P450 2E1 genotype and chlorzoxazone metabolism in healthy and alcoholic Caucasian subjects. Pharmacogenetics 5:298–304 (1995). 16. Kim, R. B., and D. O’Shea. Interindividual variability of chlorzoxazone 6-hydroxylation in men and women and its relationship to CYP2E1 genetic polymorphisms. Clin. Pharmacol. Ther. 57:645–655 (1995). 17. Johansson, I., E. Lundqvist, L. Bertilsson, M. L. Dahl, F. Sjo¨qvist, and M. Ingelman-Sundberg. Inherited amplification of an active gene in the cytochrome P450 CYP2D locus as a cause of ultrarapid metabolism of debrisoquine. Proc. Natl. Acad. Sci. USA 90:11825–11829 (1993). 18. Johansson, I., M. Oscarson, Q. Y. Yue, L. Bertilsson, F. Sjo¨qvist, and M. Ingelman-Sundberg. Genetic analysis of the Chinese cytochrome P4502D locus: characterization of variant CYP2D6 genes present in subjects with diminished capacity for debrisoquine hydroxylation. Mol. Pharmacol. 46: 452–459 (1994). 19. Clot, P., E. Albano, E. Eliasson, M. Tabone, S. Arinco`, Y. Israel, C. Moncada, and M. Ingelman-Sundberg. Cytochrome P4502E1 (CYP2E1) hydroxyethyl radical adducts as the major antigenic determinants for

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model, it is apparent that both amino acid exchanges are located in the b1-sheet, which implies that they are closely related in space. However, until detailed models or crystal structures are available, the precise role of these residues will remain unknown. Interestingly, Arg76 is conserved in all species investigated thus far [namely, human (31), macaque (32), rat (31), mouse (33), rabbit (34), and hamster (35)], which indicates an important function for this residue. This is in agreement with our data, which show altered expression of functional enzyme in the mutated variant. Val389 is also well conserved, but in the macaque, isoleucine has replaced valine, which is the same amino acid exchange found in the CYP2E1*3 allele. In line with an assumption that such an exchange would not affect the function of CYP2E1, our expression data confirm the lack of functional importance of this amino acid exchange. Our sequence analysis indicates that the flanking regions of the human CYP2E1 gene are highly polymorphic. In specific areas, up to 5% of all bases were different between the DraI C allele and the wild-type allele (see Fig. 1). An increased rate of transcription of the CYP2E1 gene has been shown to occur in rats at high ethanol concentrations (36), although the primary level for regulation of CYP2E1 in this species by ethanol is at the post-translational level (37, 38). In a preliminary study, Lucas et al. (15) found that human subjects differ with respect to inducibility of the CYP2E1 enzyme by ethanol. The extent of inducibility was lower among subjects of the c2 and DraI C genotypes. In other studies, however, the c2 allele has been shown to be more effectively expressed than the c1 allele in transfected HepG2 cells (26). Nevertheless, accumulating data suggest the occurrence of two populations of humans that are of high and low CYP2E1 ethanol inducibility,3 and it is plausible that the cause of these differences can be found at some additional polymorphic sites in the flanking regions of the CYP2E1 gene, a hypothesis supported by the present finding of a high number of mutations in the DraI C allele. Further studies are needed to resolve this question. It is interesting to note the high number of mutations in the flanking regions of the DraI C allele compared with the wild-type (DraI D) allele. By contrast, the almost complete absence of functional mutations in the open reading frame in both Caucasian and Asian populations indicates a selection for preservation of alleles encoding enzymes with the conserved amino acid sequence. Furthermore, the only functionally important mutation found did not abolish the activity of the enzyme, which further stresses the importance of the gene product. Thus, it is conceivable that CYP2E1 is of high physiological importance for humans. One might assume that a major factor in the past has been its ability to participate in the minor acetone-involving gluconeogenetic pathway (3) and that mutated CYP2E1 genes have not been beneficial for survival. However, no alteration in physiological function by homozygous inactivation of this gene was observed in well-fed mice (39). Because these mice have not been stressed dietarily, the caloric restriction selection theory for preservation of a functionally intact CYP2E1 gene in humans is not contradictory to the findings in the knock-out mice.



20. 21.




26. 27.

28. 29. 30.

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Genetic Polymorphism of Human CYP2E1 - Molecular Pharmacology

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