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TOXICOLOGY
Department of Molecular Biosciences, School of Veterinary Medicine, University of California, Davis, California
Received August 1, 2004; accepted October 26, 2004.
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Abstract |
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). The results of the National Toxicology Program 2-year inhalation studies in mice and rats have found naphthalene to be associated with neoplasia in both species. The lifetime inhalation studies in mice demonstrated slightly increased incidences of alveolar/bronchiolar adenomas only in females at the highest concentration (30 ppm) (National Toxicology Program, 1992). In rats, however, neoplasms were confined to the nasal respiratory epithelium and the incidences were concentration-dependent (National Toxicology Program, 2000). Inhalation of naphthalene vapor at levels of 2 ppm and above leads to necrosis of murine pulmonary bronchiolar epithelial cells (West et al., 2001). This exposure concentration is considerably lower than the current Occupational Safety and Health Administration standard (10 ppm, 8-h time-weighted average). These and other data were employed in the International Agency for Research on Cancer (IARC) classification of naphthalene as a possible human carcinogen (IARC Working Group, 2002). Like naphthalene, 1-nitronaphthalene (1-NN) poses a potential threat to human health. 1-Nitronaphthalene is generated in the atmosphere as a gas phase reaction product from naphthalene and N2O5. Furthermore, the nitro- and methylnitronaphthalenes are thought to account for a major fraction of the mutagenic potential associated with air toxicants in the southern California air basin (Grosovsky et al., 1999). The extent to which naphthalene and 1-NN are found in the environment, the likelihood of human exposure, and the body of evidence demonstrating toxicity in animal models support the need to understand the mechanisms of toxicity for these compounds.
Naphthalene is metabolized to naphthalene 1,2-epoxide, a reactive intermediate, by the P450 system. Both the 1S,2R- and the 1R,2S-stereoisomers are produced. This biotransformation is the first and obligate step in the cascade of events leading to injury. Microsomes or airway explants from lungs of mice metabolize naphthalene with a high degree of stereo-selectivity with ratios of 1R,2S- to 1S,2R-epoxide of 10:1 and >25:1, respectively (Buckpitt et al., 1992, 1995). Consistent with the lack of observable in vivo respiratory tract injury, both the absolute rate and the degree of stereoselectivity of naphthalene epoxidation are significantly less in rats than in mice. In contrast to the species selective toxicity observed with naphthalene, 1-NN is a potent lung toxicant in both mice and rats. P450-mediated bioactivation is essential to the toxicity of 1-NN (Verschoyle et al., 1993). Incubations of lung microsomal proteins from mice and rats display strikingly similar abilities to generate epoxides of 1-NN with the 7,8-epoxide predominating (Watt and Buckpitt, 2000).
Previous work demonstrated the presence of CYP2F2 in murine Clara cells correlates with the stereoselectivity and rate of naphthalene metabolism and with the site of injury (Buckpitt et al., 1995). Coincubation of an inhibitory CYP2F2 antibody dramatically decreases the formation of the 1R,2S- naphthalene oxide in murine lung microsomal incubations (Nagata et al., 1990). Recombinant CYP2F2 (rCYP2F2) metabolizes naphthalene rapidly and stereoselectively to the 1R,2S isomer, strongly suggesting the generation of this metabolite to be an important determinant of susceptibility (Shultz et al., 1999). In addition, rCYP2F2 metabolized 1-NN with a higher Km and lower Vmax than naphthalene; Km and Vmax values for 1-NN were 21 µM and 17 min-1, respectively. 1-NN-7,8-Epoxide was the predominate metabolite generated (Shultz et al., 2001). These data demonstrate the role of CYP2F in the initial bioactivation of these compounds. Given that rats and mice have comparable phase II detoxification systems (Lorenz et al., 1984), this unique combination of species susceptibilities are potentially attributable to 1) differences in the catalytic activities between mouse and rat CYP2F orthologs, 2) species differences in cellular CYP2F expression levels, or 3) a combination of these two factors.
Recent quantitative immunomapping studies of respiratory tract CYP2F expression have demonstrated profound differences between mice and rats correlating both with rates of in vitro naphthalene metabolism and with airway selective susceptibility (Baldwin et al., 2004). Although these results provide a reasonable explanation for differences in susceptibility to naphthalene-induced injury in rats and mice, they do not exclude the possibility that large catalytic activity differences may play a role as well. Studies comparing the metabolism of 3-methylindole by CYP2F orthologs from goat (CYP2F3) and human (CYP2F1) showed striking interspecies differences in catalytic activities of these proteins (Wang et al., 1998; Lanza et al., 1999). Similarly, recent work comparing the catalytic activities of recombinant mouse (rCYP2F2), goat (rCYP2F3), and rat (rCYP2F4) in the metabolism of dichloroethylene demonstrated relatively large differences in Km and Vmax values (Simmonds et al., 2004). To compare directly the capabilities of mouse and rat CYP2F isoforms to generate naphthalene and 1-nitronaphthalene epoxides, we have cloned and expressed a CYP2F isoform from rat lung (CYP2F4) using a baculovirus expression system. Furthermore, efforts to express rCYP2F1 (human) using systems identical to those used to generate catalytically active rCYP2F2 and rCYP2F4 yielded a recombinant protein with no apparent incorporation of heme and little capacity to metabolize naphthalene.
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Materials and Methods |
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Reagents. The mouse CYP2F2 cDNA clone in pBluescript SK- was a gift from Dr. J. Ritter (Medical College of Virginia, Richmond, VA). Recombinant CYP2F2 was previously produced in our laboratory (Shultz et al., 1999). Spodoptera frugiperda (Sf9) and Trichoplusia ni (Tn5) cells were obtained from American Type Culture Collection (Manassas, VA) and Invitrogen (Carlsbad, CA), respectively. Ex-Cell 405 medium was purchased from JRH Biosciences (Lenexa, KS). Rat NADPH cytochrome P-450 oxidoreductase (reductase) was purified from rat liver using standard procedures (Strobel and Dignam, 1978). Reductase was quantified by the standard cytochrome c reduction assay (Guengerich, 1994). Glutathione S-transferase (GST) from mouse liver cytosol was purified by standard procedures using affinity column chromatography (Simons and Vander Jagt, 1981), and activities were assessed with 1-chloro-2,4-dinitrobenzene as substrate. Unless otherwise stated, all other reagents were purchased from commercial vendors and were of reagent/analytical grade.
Construction of Rat Lung cDNA Library and Isolation of Rat CYP2F4. Lungs from four rats were perfused with saline, quickly removed, and then flash frozen in liquid nitrogen. Frozen sections of approximately 100 mg were used to isolate total RNA (RNeasy Mini; QIAGEN, Valencia, CA) from each rat. Total RNA was pooled, and poly(A)+ RNA was affinity purified on an oligo(dT)-cellulose column. Prior to cDNA library construction, 3 µg of poly(A)+ RNA was subjected to northern blot analysis using a 32P-labeled cDNA probe containing approximately 1400 bp of the mouse CYP2F2 open reading frame (ORF) to verify the presence of a cross hybridizing transcript of the appropriate length in rat lung (results not shown). Double-stranded cDNA was synthesized from poly(A)+ RNA and directionally ligated to the bacteriophage vector 
ZAP using a cDNA synthesis kit (ZAP-cDNA synthesis kit; Stratagene, La Jolla, CA). Recombinant phage-infected XL1-Blue MRF' cells were screened with the 32P-labeled cDNA probe used previously for northern analysis, and pBluescript phagemid was excised from positive plaques. Using a combination of restriction digestion and direct sequencing (Applied Biosystems, Foster City, CA), several clones were found to contain cDNA from a CYP2F2 ortholog, two of which contained the entire ORF. The two full-length clones were bidirectionally sequenced and the consensus sequence (CYP2F4) was submitted to the P450 nomenclature committee and then GeneBank (accession no. AF017393
[GenBank]
).
Expression of Recombinant CYP2F4 and CYP2F1. The cDNA insert encoding rat CYP2F4 (0–1776 bp) was excised from pBluescript SK-using the EcoRI and XhoI cleavage sites and directionally cloned into the multiple cloning site of pFastBac1 (Invitrogen). The integrity and orientation of the pFastBac/2F4 clone was verified by bidirectional sequencing. The cDNA encoding CYP2F4 from pFastBac1/2F4 was site-specifically transposed into the baculovirus genome as described in the manufacturer's protocol (Bac-to-Bac Expression System; Invitrogen). The high molecular weight genomic DNA was purified from recombinant clones and used to transfect Sf9 cells for the production of baculovirus stocks.
Human lung tissue was obtained via Golden State Organ Donor Services (Sacramento, CA) and used to isolate total RNA (RNeasy Mini; QIAGEN). To clone the CYP2F1 ORF, RNA was reverse-transcribed (Superscript II; Invitrogen) using a poly(A) primer followed by PCR amplification (Turbo PFU; Stratagene) of the single-stranded cDNA using a forward primer containing a BclI cleavage site (5'-gggcgctgatcaaccATGgacagcataagcacag-3') and a reverse primer containing a HindIII cleavage site (5'-atcgtaaagcttgTTAgcgcgggcgcagg-3'). The PCR product was purified (QIAquick PCR purification kit; QIAGEN), restriction digested with BclI and HindIII, and then directionally cloned into the BamHI and HindIII sites of the pFastBac1 transfer vector multiple cloning site. The cloned CYP2F1 cDNA was bidirectionally sequenced and found to be identical to the CYP2F1 mRNA RefSeq (NM_000774 [GenBank] ). Recombinant CYP2F1 baculovirus stocks were prepared in an identical fashion to CYP2F4.
Baculovirus stocks were amplified in Sf9 cells and viral titer was obtained using a BacPAK Baculovirus Rapid Titer kit (BD Biosciences Clontech, Palo Alto, CA). Tn5 cells grown as monolayers in complete Ex-Cell 405 were used to optimize expression and produce active enzyme. Infections were performed by incubating virus with the cells in the presence of 100 µM 5-aminolevulinic acid (ALA) and 100 µM ferric citrate (FC). Cell lysates were prepared by pelleting cells at 1000g for 10 min followed by three washes with ice-cold phosphate-buffered saline and resuspension in 0.1 M phosphate buffer, pH 7.4, with 20% glycerol and protease inhibitors (Cocktail Set III; Calbiochem, San Diego, CA). Cells were lysed with two 10-s rounds of sonication on ice followed by centrifugation at 1000g for 10 min to remove unlysed cells. When spectrally active recombinant protein was obtained, cell lysate spectral activity per milligram of protein was used as an endpoint to optimize multiplicity of infection and viral incubation time. P450 levels were determined by obtaining difference spectra of sodium dithionite-reduced versus CO-bubbled samples at 500 to 400 nm according to Omura and Sato (1964). Alternatively, in the case of CYP2F1 where spectrally active protein was unobtainable, immunoblot analysis was used as a surrogate endpoint. Proteins from Tn5 cell lysates were separated by SDS-polyacrylamide gel electrophoresis using 1-mm 10% BisTris gels (Invitrogen). Bands were visualized by SYPRO Ruby staining (Molecular Probes, Eugene, OR). To determine relative protein abundances, SYPRO Ruby-stained gels were scanned on a Typhoon 8600 scanner, using a 532-nm excitation wavelength and a 610BP30 emission filter. Immunoblots using a rabbit polyclonal anti-CYP2F2 antibody (Nagata et al., 1990) were performed as described previously (Baldwin et al., 2004).
To serve as a positive control during rCYP2F1 expression studies, rCYP2F4 viral stocks were used concurrently, and reagents were pooled wherever possible. To address the possibility that rCYP2F1 was more labile than rCYP2F4, a subpopulation of viral-infected Tn5 cells were harvested and lysed using only glass-glass homogenization without sonication. Additionally, after the Tn5 cells were centrifuged to harvest recombinant protein, DNA was isolated (Plasmid Mini kit, QIAGEN) from an aliquot of the virus-containing cell culture media supernatant. Using primers flanking the transposition site in the viral genome (M13 forward and reverse), the transposed pFastBac1 sequence was PCR amplified using a polymerase with high fidelity and processivity (Herculase; Stratagene). After removal of unincorporated nucleotides and primers (QIAquick PCR purification kit; QIAGEN) the 
1500 base region containing either the CYP2F1 or CYP2F4 ORF within the 4-kilobase amplicon was sequenced to verify the gene sequence of the CYP2F baculoviruses and to rule out the possibility of viral cross contamination.
Measurement of Naphthalene and 1-Nitronaphthalene Metabolism. The rates of naphthalene metabolism were determined in incubations containing recombinant CYP2F4 (quantity determined spectrally), reductase (quantified by cytochrome c activity), NADPH-regenerating system (0.25 U glucose-6-phosphate dehydrogenase, 14 mM glucose 6-phosphate, 2.18 mM NADP, and 1 mM MgCl2), 1 mM glutathione, GST (amount specified in figure legends), and 2 mM CHAPS in a total volume of 250 µl (0.1 M Na2HPO4, pH 7.4). The ratio of reductase to CYP2F4 (units/picomole) as well as the concentration of CHAPS detergent were optimized for greatest enzyme activity for each substrate and used for all kinetic determinations. Glutathione and GST were included for the trapping of reactive epoxides as stable glutathione conjugates. Enzyme incubations and the separation of glutathione conjugates by reversed-phase HPLC with quantification by UV absorption were performed as described previously (Shultz et al., 1999).
Using conditions optimized for maximal naphthalene turnover with rCYP2F4, the activity of Tn5 cell lysates containing rCYP2F1 was studied. Cell lysates and cofactors were incubated with 1 mM naphthalene at 37°C for 20 min. Given the absence of spectral activity, comparisons of rCYP2F1 and rCYP2F4 naphthalene metabolism were standardized based on total amounts of cell lysate protein in each incubation. Similar levels of immunoreactive CYP2F per milligram of cell lysate protein for both isoforms justified this approach (Fig. 1, B and C). Given the anticipated low or nonexistent levels of naphthalene metabolism, lysates from both noninfected and wild-type baculovirus-infected Tn5 cells were used as negative controls. Additionally, in several enzyme incubations the amount of reductase was varied independently as a means to rule out any metabolic contribution arising from the reductase preparation.
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Incubations with 1-NN were carried out in 250-µl volumes with amounts of recombinant CYP2F4, reductase, and other cofactors optimized for maximal 1-NN turnover as described above. Glutathione conjugates were separated by HPLC and measured by UV absorption at 256 nm according to established methods (Watt et al., 1999). Quantification of 1-NN conjugates was based on the preparation of 14C-labeled standards. [14C]1-NN (1 mM) was incubated with rat liver microsomes for 10 min at 37°C. Methanol extracts of the incubation mixture were evaporated to dryness and reconstituted for HPLC analysis. Fractions of the column eluate were collected at 15-s intervals and radioactivity counted with a Beckman LS5000TD scintillation counter. Peak areas at 256 nm for each of the metabolite peaks were compared with total disintegrations per minute for the peak to obtain peak area per nanomole ratios. These ratios were subsequently used to determine metabolite quantities in incubations with unlabeled substrate.
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1900 bp was found to hybridize with a mouse CYP2F2 probe under stringent conditions (data not shown). Accordingly, the rat ortholog of CYP2F2 was cloned from a lung cDNA library. The consensus sequence of the novel gene derived from two full-length clones was 1768 bp and contained 12 bp of 5'UTR. The deduced amino acid sequence of CYP2F4 (accession no. AF017393
[GenBank]
) showed a homology of 94% with CYP2F2 and 81% to CYP2F1. This novel P450 was then expressed in insect cells using the baculovirus expression system. As in previous work, Tn5 cells were found to yield higher amounts of recombinant protein compared with Sf9 cells. A major cellular protein with an apparent molecular weight of 50 to 52 kDa was present in lysates of Tn5 cells infected 84 h earlier with baculovirus containing CYP2F4 (Fig. 1A). Immunoblot analysis of lysate proteins confirmed the presence of a protein recognized by a polyclonal antibody generated to CYP2F2, comigrating with the immunoreactive band observed in rat terminal bronchioles (Fig. 1B). A typical yield of spectrally active CYP2F4 was 260 pmol/mg cell lysate protein. Incubation of Tn5 cells with the CYP2F1 baculovirus produced significant amounts of recombinant protein as visualized in SYPRO Ruby-stained gels (Fig. 1A). Immunoblot analysis of Tn5 cell lysates and microsomes prepared from the rhesus macaque ethmoid nasal epithelium, the respiratory tract subcompartment with the greatest CYP2F abundance, using an antibody generated to CYP2F2 demonstrated comigration of immunoreactive proteins (Fig. 1B). Comparable amounts of immunoreactive rCYP2F1 and rCYP2F4 apoprotein were produced in Tn5 cells infected in parallel when data were normalized per nanogram of cell lysate protein (Fig. 1C). Multiple experiments demonstrated CO-difference spectra for ALA/FC supplemented rCYP2F1 which were not discernibly different from spectra obtained from lysates of supplemented noninfected cells (Fig. 2). Substitution of glass-glass homogenization for sonication of cell pellets from either CYP2F4 or CYP2F2 baculovirus-infected cells resulted only in a significant decrease in the amount of immunoreactive CYP2F protein per milligram of cell lysate protein and in the case of rCYP2F4, a reduction in P450 levels determined spectrally. Sequence analysis of CYP2F1 and CYP2F4 baculoviruses during expression demonstrated the absence of any mutations.
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Measurement of Naphthalene and 1-Nitronaphthalene Metabolism. Prior to the determination of the catalytic activity of rCYP2F4, incubation conditions and cofactor concentrations were optimized for maximal naphthalene turnover as described previously for rCYP2F2 (Shultz et al., 1999). The concentration of detergent (CHAPS) in the incubation was found to significantly affect the rate of naphthalene metabolism; increasing the CHAPS concentration to 8 mM resulted in a precipitous, 70% reduction in maximal enzyme activity (Fig. 3). Based on these results, a concentration of 2 mM was used for all further studies. Preliminary studies directly comparing catalytic activities of rCYP2F4 and rCYP2F2 using saturating naphthalene concentrations (0.5–1.0 mM) revealed nearly identical maximal catalytic activities and stereoselectivities (data not shown). For further studies with rCYP2F4, the linearity of product formation with incubation time and enzyme concentration was determined, and all incubations were conducted in the linear portions of these curves. Incubations were performed for either 4 or 6 min using substrate concentrations ranging from 2 µM to 2 mM. Reciprocals (1/v versus 1/S) were plotted, and intercepts were calculated by linear regression analysis (Fig. 4). Values for Km and Vmax are shown in Table 1. The ratio of 1R,2S/1S,2R epoxides inferred from the glutathione conjugates was >50:1.
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Incubations of naphthalene with rCYP2F1 yielded rates of naphthalene metabolism per milligram of cell lysate protein ranging from 100- to 900-fold less than identical incubations using rCYP2F4. Activities with rCYP2F1 were never statistically different from those of either negative control (Table 2). Although the differences were not statistically significant, it appeared that total naphthalene metabolism was more sensitive to changes in the amount of reductase than to the amount of recombinant CYP2F1 protein (Table 2). A metabolism scheme along with representative chromatograms of extracts prepared from incubations of rCYP2F1 and rCYP2F4 with naphthalene are shown in Fig. 5. Based on our inability to detect any metabolic activity associated with rCYP2F1, no further metabolic studies were performed with rCYP2F1.
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Assay conditions, cofactors, and linearity with time and enzyme concentration were independently optimized with CYP2F4 for maximal turnover of 1-NN. Incubations were conducted for 10 min at substrate concentrations of 2 to 200 µM. Recombinant CYP2F4 metabolized 1-NN to both the 5,6- and 7,8-epoxide intermediates that were trapped and quantified as glutathione conjugates. The identity of these metabolites was established by comigration with purified standards whose identity and regiochemistry were established by mass spectroscopy and NMR (Watt et al., 1999). Figure 6 shows the structures and scheme of 1-NN metabolism, as well as the corresponding peaks on HPLC. The predominant conjugates detected were metabolites 1, 2, 3, 4, and 6 corresponding to a 20:1 ratio of 7,8-epoxide to 5,6-epoxide. The Km and Vmax for the conversion of 1-NN to glutathione conjugates are shown in Table 1.
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). These species differences in susceptibility correlate well with the rate of metabolism of naphthalene to epoxides in both lung microsomes (Buckpitt et al., 1992) and in dissected airway explants (Buckpitt et al., 1995). Furthermore, there are no striking differences in either pulmonary epoxide hydrolase- or GST-mediated detoxification pathways for naphthalene oxide, which would account for the unusual susceptibility of the mouse compared with the rat (Lorenz et al., 1984). Generation of naphthalene oxide, the first and obligate step in the cascade of events leading to injury, is mediated by CYP2F, making this enzyme a key factor in the species susceptibility of this compound (Warren et al., 1982; Ritter et al., 1991). The observed differential in rates of naphthalene activation across species and within the respiratory tract is likely attributable to differences in CYP2F expression, catalytic activity, or a combination of both factors. Recombinant mouse CYP2F2 generates naphthalene oxide with high catalytic efficiency and stereoselectivity, supporting its role in the generation of reactive metabolites in this species (Shultz et al., 1999). Recent quantitative immunoblot studies showed significant differences in CYP2F expression between mice and rats (Baldwin et al., 2004). These findings are consistent with the view that enzyme expression accounts, at least partially, for differences in susceptibility to naphthalene toxicity. The current work revealed that rat CYP2F4 generates naphthalene and 1-NN epoxides with catalytic activities and stereoselectivities nearly identical to the mouse isoform. These findings indicate that CYP2F expression is closely associated with susceptibility to naphthalene-induced injury and that limited expression of CYP2F is sufficient to confer resistance in rats. Studies of heterologously expressed CYP2F1 demonstrated significant yields of immunoreactive, yet spectrally inactive, recombinant protein thus suggesting the generation of the apoprotein but not the holoenzyme. As expected, this protein had only a very limited ability to catalyze the conversion of naphthalene to naphthalene-oxide, indiscernible from negative controls.
If CYP2F4 were a major contributor to the metabolism of naphthalene in vivo, then the catalytic activity and high degree of stereoselectivity for naphthalene epoxidation demonstrated by rCYP2F4 should be reflected by high substrate turnover and high ratios of 1R,2S- to 1S,2R-epoxide within the respiratory tract. Airway subcompartments microdissected from rat lung generate naphthalene oxide at relatively low rates and the 1S,2R-epoxide is the major metabolite. These data indicated a negligible contribution from CYP2F4 in these areas of the respiratory tract (Buckpitt et al., 1995). Data obtained with rat nasal epithelium is strikingly different, displaying significant naphthalene turnover with more than a 30-fold ratio of 1R,2S- to 1S,2R-epoxide in the olfactory epithelium (Buckpitt et al., 1992). The highest rates of naphthalene turnover were found in the olfactory epithelium, followed by the lateral wall (2-fold less) and the septum (9-fold less). Immunoblot studies quantitating the relative differences in CYP2F4 expression within the rat respiratory tract have defined a distribution pattern nearly identical to the patterns of 1R,2S generation (Baldwin et al., 2004). These data suggest that CYP2F4 expression is proportional to 1) the amount of 1R,2S-epoxide generated, and 2) the extent of naphthalene-induced injury observed in vivo. Therefore, the most important factor in determining tissue susceptibility to naphthalene injury in the rat appears to be the level of CYP2F4 expression.
Previous studies in mice and rats using 1-NN have demonstrated similar in vivo cytotoxicities (Rasmussen et al., 1986; Sauer et al., 1997). Furthermore, in vitro incubations of lung microsomal proteins have shown strikingly similar rates of substrate epoxidation with the 7,8-epoxide predominating in both species (Watt and Buckpitt, 2000). Prior characterization of rCYP2F2 and the preponderance of 1-NN glutathione conjugates 2 and 4 (arising from the 7,8-epoxide) in mouse lung incubations supports the involvement of CYP2F2 in the metabolism of 1-NN in this tissue, a finding that is consistent with recent immunoblot studies (Baldwin et al., 2004). Conversely, the current studies showing rCYP2F4 to strongly favor the generation of 1-NN glutathione conjugates 2 and 4 and the nearly equal amounts of 1-NN glutathione conjugates 1, 3, and 4 (from both 5,6- and 7,8-epoxides) observed in lung microsomal incubations support the involvement of other P450 isoform(s) in the bioactivation of 1-NN in the lungs of rats. These findings are consistent with the conclusions of Verschoyle and coworkers who suggested that the bioactivation of 1-NN were catalyzed by CYP2B in rat lung (Verschoyle et al., 1993).
Data on CYP2F1 expression in human tissue are limited with the majority of studies utilizing reverse transcriptase-PCR techniques to detect CYP2F1 transcript. With the exception of the lung and placenta, all other human tissues tested have no detectable levels of CYP2F1 mRNA (Hakkola et al., 1996; Andersen et al., 1998; Nishimura et al., 2003). Assessment of CYP2F1 transcript levels in the respiratory tract has been limited to homogenates of whole lung. Therefore, expression levels within discrete areas of the conducting airways or nasal epithelium are unknown. Direct evidence for CYP2F1 protein in the human lung is also lacking, but recent work in rhesus macaques using an antibody to CYP2F2 showed undetectable amounts of protein in all segments of the respiratory tract except the ethmoid nasal epithelium (Baldwin et al., 2004). Despite an incomplete understanding of the expression of CYP2F1 in the human respiratory tract, the value of determining enzyme expression levels is contingent on the existence of a catalytically active protein.
The ability of human CYP2F1 to generate naphthalene oxide remains equivocal. Initial studies using a vaccinia-virus system to express recombinant CYP2F1 yielded small amounts of protein, necessitating 6-h incubations to detect metabolites (Thornton-Manning et al., 1996). The profile of 3-methylindole metabolites generated differed substantially from those obtained using rCYP2F3 (Wang et al., 1998). In an attempt to address these issues, Lanza et al. (1999) utilized a lymphoblastoid system to express spectrally quantifiable amounts of rCYP2F1 to further study the kinetics of 3-methylindole and naphthalene metabolism. Saturating concentrations of naphthalene (500 µM) and large amounts of rCYP2F1 (240 pmol/incubation) yielded levels of naphthalene conjugates near the analytical limit of detection with an 8-fold preference for the 1S,2R-epoxide. Maximal naphthalene turnover was 35.5 pmol/nmol P450/min or 0.036 min-1, approximately 3000-fold lower than values obtained with rCYP2F4 or rCYP2F2.
Side by side expression studies of rCYP2F1 and rCYP2F4 yielded significant amounts of both proteins, each having the appropriate molecular weight and immunoreactivity. However, only rCYP2F4 produced a detectable reduced CO-difference spectra, indicating that heme was correctly incorporated in the rodent CYP2F but not in human CYP2F1. Although there are many examples of mutations that cause loss of function in human P450 isoforms (reviewed in Ingelman-Sundberg, 2002; http://www.imm.ki.se/CYPalleles/), the majority of these alterations are due to large deletions or point mutations causing splice-site, frameshift, or nonsense mutations and hence a protein product with an altered molecular weight. Given the multiple rounds of sequence verification, a mutation in the expressed CYP2F1 is unlikely. Several studies using heterologously expressed human P450 alleles containing a single missense mutation have demonstrated a complete loss of function as evidenced by the absence of both spectral and metabolic activity (Yamano et al., 1990; Evert et al., 1997). However, the precedent does exist for baculovirus-expressed P450 proteins to have no detectable CO-difference spectrum, yet measurable catalytic activity. Even though the spectrally inactive CYP2A6*6 allele is only 10% as active in coumarin hydroxylation as its wild-type counterpart, these activities were still well above (10-fold) controls (Kitagawa et al., 2001). This does not appear to be the case with CYP2F1 where detectable metabolic activities were indiscernible from negative controls.
As indicated earlier, previous studies in a lymphoblastoid expression system (Lanza et al., 1999) were able to measure small amounts of cytochrome P450 (20 pmol/mg microsomal protein). More recent studies, which used a cytomegalovirus-based viral vector to express CYP2F1 in a human bronchial epithelial cell line (BEAS-2B), have demonstrated the presence of recombinant protein by immunoblot analysis (Nichols et al., 2003; Sheets et al., 2004). Both studies demonstrated rCYP2F1 catalytic activity in BEAS-2B cells, inferred by either loss of cell viability with 3-methylindole incubation or quantification of benzene metabolism. Benzene metabolism was relatively limited with an estimated Vmax of 10 pmol/nmol P450/min. Thus, from the available data 1) functional CYP2F1 has been difficult to express, 2) rCYP2F1 does not incorporate heme properly in a baculovirus system which yields high levels of catalytically active rodent CYP2F proteins, and 3) when rCYP2F1 holoenzyme is expressed, relatively low rates of substrate metabolism are observed.
In summary, the data presented here demonstrate that rat rCYP2F4 metabolizes naphthalene and 1-NN with high catalytic activities and regioselectivity, nearly identical to mouse rCYP2F2. Therefore, the observed differences in species and respiratory distribution patterns of 1R,2S-epoxide generation and in vivo cytotoxicity are likely due to differences in levels of CYP2F expression. Low expression levels of CYP2F protein are sufficient to account for the insensitivity of rats to naphthalene-induced cytotoxicity. Extrapolation of these findings to humans and other primates would suggest that, given equally efficient phase II detoxification systems (Pacifici et al., 1981; Bryan and Jenkinson, 1987), a deficit in either CYP2F catalytic activity or expression levels would result in an insensitivity to naphthalene-induced injury. Although relative expression data exist for the rhesus macaque, analogous data in the human is lacking. Future immunologic and/or proteomic studies could provide these comparative data. In addition, characterization of the multiple potential human CYP2F1 alleles identified from public genetic databases, along with CYP2F1/2F4 chimeras, should prove beneficial in determining regions critical in the expression of catalytically active protein.
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Acknowledgements |
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Footnotes |
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Article, publication date, and citation information can be found at http://jpet.aspetjournals.org.
ABBREVIATIONS: 1-NN, 1-nitronaphthalene; P450, cytochrome P450; rCYP2F, recombinant CYP2F; GST, glutathione S-transferase; bp, base pair(s); ORF, open reading frame; PCR, polymerase chain reaction; ALA, 5-aminolevulinic acid; FC, ferric citrate; CHAPS, 3-[(3-cholamidopropyl)dimethylammonio]-1-propanesulfonate; HPLC, high-pressure liquid chromatography; CDNB, 1-chloro-2,4-dinitrobenzene.
Address correspondence to: R. Michael Baldwin, Veterinary Medicine: Molecular Biosciences, 1311 Haring Hall, UC Davis, Davis, CA 95616. E:mail: rmbaldwin{at}ucdavis-alumni.com
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References |
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