Bioavailability and biotransformation of benzo(a)pyrene in an isolated perfused In situ catfish intestinal preparation.

In the aquatic environment, diet is an important route of exposure for the common contaminant and procarcinogen benzo(a)pyrene (BaP). Dietary organisms vary in their BaP content and in contaminated areas often contain other xenobiotics including cytochrome P4501A inducers. This study examined the effect of dose and previous dietary exposure to the inducer ss-naphthoflavone (BNF) upon the intestinal metabolism of BaP and the systemic bioavailability of BaP-derived products in catfish. BaP was administered at 2 and 20 microM into in situ-isolated perfused intestines of control and BNF-pretreated catfish. The intestine formed an array of metabolites in all treatments including potentially hazardous metabolites such as BaP-7,8 and 9,10 dihydrodiols and 6-methyl-BaP. BNF treatment disproportionally increased the contribution of BaP-7,8 and 9,10 dihydrodiols relative to the contributions of other metabolites. A greater percentage of metabolites was evident as conjugates in 2 microM controls, whereas a greater percentage of unconjugated metabolites was evident for 20 microM controls and BNF treatments of both dosages. BNF pretreatment and the higher 20 microM BaP dosage resulted in greater bioavailability, with 2.6-5.5-fold and 3.0-6. 3-fold increases in systemically available BaP products, respectively. Metabolites represented 10.2-23.1% of the increased bioavailability with BNF treatment, suggesting that mechanisms, in addition to induced metabolism, may be operative. These results indicate that intestinal bioavailability, level of biotransformation, and the metabolic profile of BaP-derived products entering the blood from the intestine may be altered by dose and dietary BNF pretreatment.

In the aquatic environment, diet is an important route of exposure for the common contaminant and procarcinogen benzo(a)pyrene (BaP). Dietary organisms var'yin their BaP content and in contaminated areas often contain other xenobiotics including cytochrome P4501A inducers.
This study eamined the effect of dose and previous dietary exposure to the inducer 3-naphthoflavone (BNF) upon the intestinal metabolism of BaP and the sptemic bioavailability of BaP-derived products in catfish. BaP was administered at 2 and 20 pM into in situ-isolated perflsed intestines of control and BNF-pretreated catfish. The intestine formed an array of metabolites in all treatments including potentially hazardous metabolites such as BaP-7,8 and 9,10 dihydrodiols and 6-methy-BaP. BNF treatment disproportionally increased the contribution of BaP-7,8 and 9,10 dihydrodiols relative to the contributions of other metabolites. A greater percentage of metabolites was evident as conjugates in 2 pM controls, whereas a greater percentage of unconjugated metabolites was evident for 20 pM controls and BNF treatments of both dosages. BNF pretreatment and the higher 20 pM BaP dose resulted in greater bioavailabilit4 with 2.6-5.5-fold and 3.0-6.3-fold s in temically avhlable BaP products, respectively.
Metabolites represented 10.2-23.1% of the increased bioavilability with BNF treatment, saggesting that mechanisms, in addition to induced metabolism, may be operative. These results indicate that intestnal bioavailability, level of biotransformation, and the metabolic profile of BaP-derived products entering the bloed from the intestine may be altered by dose and dietary BNF pretreatment. Key wordk: activation, benzo(a)pyrene; bioavailability, biotransformation, catfish, eimination, in situ preparation, intestine. Environ Health Perspect 106:155-166 (1998).
[Online 5 February 1998] httap://ehpnedt.niess.nih.govldocs/A998/106p155-166kkinow/abaract.html Polynuclear aromatic hydrocarbons (PAHs) are frequently found as contaminants in impacted aquatic environments. These compounds have been associated with areas that demonstrate a high tumor prevalence in wild fish populations (1)(2)(3). The carcinogenicity of PAHs is a well-known consequence of their metabolic activation (4). Among the various PAHs, the model compound benzo(a)pyrene (BaP) has received the most attention in fish species, with a primary focus on hepatic metabolism and adduct formation (5,6). BaP has been shown experimentally to be carcinogenic to fish following both waterborne (7) and oral exposures (8).
The hydrophobicity and environmental partitioning (9) of BaP, as well as its accumulation in infaunal invertebrates (10,11), suggest that the diet may be an important route of exposure for aquatic species.
Studies examining various levels in the aquatic food chain have demonstrated not only the presence of BaP in diet and tissues but the biotransformation of BaP by lower organisms and the subsequent food chain transfer of BaP molar equivalents (Meq) to higher organisms (12)(13)(14). (BaP molar equivalent is defined here as BaP and BaPderived metabolites compositely quantified by radioactivity and placed on an equal molar basis using BaP's specific activity.) Dietary BaP may also undergo biotransformation by the intestine of the consumer before entering the systemic circulation (15). Intestines of fish are capable of a wide variety of biotransformation reactions, some of which respond to dietary cytochrome P4501A (CYPIA) inducers (16). Dietary induction studies in both flounder (17) and catfish (16) indicate that under conditions of low inducer concentrations, select biotransformation activities in the intestine may equal or even exceed corresponding hepatic activities. Such induction effects may potentially alter the degree and pathway of metabolism. Similarly, in vitro BaP studies with flounder intestinal homogenates suggest that the biotransformation pathways and products formed in the intestine may be altered by the BaP dose (17). BaP may be activated or alternatively detoxified by metabolically favored pathways. These findings suggest that the balance between toxification and detoxification on first-pass metabolism through the intestine may depend on dose and previous exposure history.
Objectives of the present study were to examine the intestinal metabolism and bioavailability of BaP in context of the products formed under varying conditions of dose and previous exposure history. These goals were addressed using an in situ isolated perfused intestinal model (catfish). BaP dosages used were based on Km determinations of relevant biotransformation enzymes in the intestine. Dietary pretreatment was accomplished using the CYPIA inducer j-naphthoflavone (BNF) at concentrations in the diet that would induce the intestine but not the liver.

Materials and Methods
Channel catfish (1,639 ± 300 g) were obtained from the Louisiana State University (LSU) Aquaculture Research Station, Baton Rouge, Louisiana. Fish for all treatment groups were maintained under flow through conditions in dechlorinated tap water (pH 8.10 ± 0.33; temperature 21.0 ± 1.1°C; total hardness 25.7 ± 7.2 mg CaCO3/l; alkalinity 170.3 ± 18.2 mg/l) on a 12-hr light photoperiod. Fish were acclimatized at least 4 weeks to experimental conditions before use. All fish were held and treated in accordance with National Institutes of Heath guidelines. Virgin Silvercup trout chow (Murray Elevators, Murray, UT) was fed to fish before experimental treatment. On initiation of experimental treatment, control fish were maintained on trout chow coated with corn oil (100 pl corn oil/100 g chow), whereas fish to be induced were fed 1 mg BNF/100 pl corn oil/100 g chow. Both dietary groups were maintained on appropriate experimental diets at 30 g feed/ kg/day for 14 days before surgical manipulation. Fish were fasted 24 hr before surgery and in situ experimentation.
Intestinal microsomes were prepared from control and BNF-exposed catfish for use in in vitro studies of BaP positional metabolism and monooxygenase Km and Vm determinations. Catfish were immobilized in ice water and sacrificed by severing the spinal cord (n = 4/treatment). Intestines were removed, rinsed thoroughly with ice-cold buffer 1 [0.25 M sucrose, 5 mM EDTA, 0.05M Tris-Cl, pH 7.4, 0.2 mM phenylmethyl sulfonyl fluoride (PMSF)] to remove contents, and cut open; mucosal cells were then removed by scraping with a scalpel. The mucosa was placed in 10 ml buffer 1 and the cells were sedimented at 2,000 x g, weighed, and homogenized in 4 vol buffer 1. Washed microsomal fractions were prepared by differential centrifugation using the procedure described by James and Little (18).
Surgical procedures. Catfish of either sex were anesthetized with buffered (NaHCO3;) tricane methane sulfonate (Argent Chemical Company, Redmond, WA) at induction and maintenance doses of 106 and 86 mg/l, respectively. On induction, individual catfish were administered 1.5 ml anticoagulant (75 mM sodium citrate:42 mM citric acid: 136 mM dextrose) and transferred to an aquatic surgery table.
The intestine was exposed by a longitudinal ventral midline incision. A ventral loop of proximal intestine starting 10 cm caudad to the pylorus and extending aborally approximately 20 cm was used for the preparation (Fig. 1). The afferent (supply) vessel, a branch of the coeliacomesenteric artery, and the corresponding efferent (drainage) vessel perfusing the prospective intestinal segment as well as potential collateral vessels were identified and isolated, and suture (00 silk) was placed loosely around each. Once ligatures were in place, blood was drawn from the caudal vein into a syringe containing citrate anticoagulant. The syringe, with a total of 10 ml blood and 1 ml oxygen (as determined by preliminary blood gas studies), was placed on an orbital mixer that provided gentle agitation for the cells.
The isolated afferent vessel was cannulated using anticoagulant-filled PE-50 (polyethylene) tubing. Once secured in place, the line was cleared, attached to a syringe pump mounted on a rocking platform, and a blood flow rate of 0.1 ml/ min was established. After cannulation of the efferent vessel with PE-60 tubing, the ligatures loosely placed around collateral vessels were rapidly tied off. Efferent blood volume was measured to ensure that blood output equaled input so as to verify that the infusion and drainage were for the isolated segment. The preparation was transiently blanched with a small amount of anticoagulant in saline through the afferent cannula. Throughout blanching, the course was examined to ensure that the afferent cannulation supplied the intestinal segment before collection in the efferent cannula; to determine the efficiency or completeness of the intestinal segment perfusion; and to demarcate the length of intestine perfused in the soon-to-be isolated intestinal segment preparation. Immediately after blanching, the region of perfusion was noted and blood flow reestablished. Ligatures were then preplaced slightly in from the perfusion margin on the intestine to mark the isolated segment.
Dose preparation and introduction. At the time of dosing, the ligature around the distal extent of the perfused isolated intestinal segment was tied off. A small sample of micelle preinfusate was then collected for verification of BaP purity at time of analysis. The needle of the dosing syringe was inserted through the gut wall and the tip of the needle extended in the gut lumen for 2 cm beyond the proximal ligature. This ligature was then tightened over the needle allowing injection of the micellar solution and BaP dose into a nonperforated isolated intestinal segment. The injected dose was gently massaged throughout the entire segment, the timer started, and the room lights turned off to minimize photolysis of BaP.
In situ intestinal preparations in select experiments were dosed with [3H]-BaP via the perfusion blood.
[3H]-BaP in an ethanol carrier was added directly to blood so that the BaP dose delivered during the timed perfusion was the same as that in the corresponding luminal study (2 pM). Once [3H]-BaP was added to the blood, the carrier vehicle was evaporated and blood was throughly mixed and loaded into a syringe for perfusion. A micelle solution of identical composition (except for BaP) and volume as that used in the luminal studies was placed in the lumen of the intestinal segment as a collection medium.
Sample collection. Throughout the course of the 60-min perfusion, the intestine was moistened with saline (as needed), blood flow was checked every 10 min, and the isolated segment was gently massaged every 5 min. Whole blood collected compositely over the 60-min perfusion was sampled at each flow check to ensure proper sample representation. At the end of the perfusion, samples of liver, kidney, and anesthetic water were taken for radioactivity analysis to check the isolated preparation's perfusion integrity. (In intact isolated preparations, no radioactivity should be present in the samples.) The isolated ligated intestinal segment was removed intact and the length measured under standardized conditions. Postinfusate was collected by draining the intestinal segment, volumes were recorded, and aliquots taken for liquid scintillation counting and metabolite analysis. Once drained, the intestinal segment was cut open along the entire length, copiously washed with saline, and blotted dry. The mucosal surface was examined grossly for viability and then scraped with a glass slide. Mucosal tissue was mixed and aliquots were taken for liquid scintillation counting (approximately 100 mg) and metabolite analysis. Preinfusate, blood, liver, kidney, water, intestinal mucosa, and postinfusate were processed for liquid scintillation counting, as described below. Samples for metabolite determination (preinfusate, postinfusate, intestinal mucosa, and blood) were placed under nitrogen, wrapped in foil, and frozen at -20°C for up to 1 month until analysis.
Radioassay procedures. Tissue and postinfusate samples (approximately 100 mg) were digested in TS-1 (0.5 ml) tissue solubilizer (Research Products International, Mount Prospect, IL) for 24 hr at 500C. After cooling, the samples were neutralized with 18 pi glacial acetic acid and counted in 4.5 Analysis. Blood, mucosal cell, and postinfusate medium samples from the [3H]-BaP-incubated in situ intestinal preparation were extracted by matrix solid phase dispersion, as described by James et al. (20). Briefly, samples of mucosal cells, 0.2-0.5 g, were added to 2 g prewashed, air-dried octadecylsilane-coated silica beads (C1 8)' 30-70 pm, (Alltech Associates, Deerfield, IL). The mixture was gently blended with a glass pestle to produce an evenly mixed, semidry material. This material, packed in a column, was eluted sequentially with 16 ml heptane and then with 8 ml each toluene, ethyl acetate, methanol, and water. Solvent eluents were collected in separate vials. After solvent elution, the packing material was extruded from the column, weighed, and mixed well. Five separate 0.1-g samples were then added to 18 ml scintillation cocktail and assayed for radioactivity. Aliquots of each solvent eluent were counted and the percentage of radioactivity in each fraction calculated. The heptane, toluene, ethyl acetate, and methanol fractions were dried separately under nitrogen, taken up in 0.25 ml 55% methanol, and filtered through a 0.45-pm centrifuge filter; the solutions were analyzed by HPLC. Selected aqueous fractions were hydrolyzed before analysis. Similar procedures were used for blood and postinfusate except that 0.2-1-ml samples of postinfusate and 3-6-ml samples of blood were used. Where sample size was greater than 0.5 ml, the amount of packing material mixed with the sample and the volume of eluent used were increased proportionally. The percentages of recovery, binding, and decomposition were determined by adding standards to mucosa, blood, and postinfusate and following the above procedure ( Table 1).
The evaporated and reconstituted heptane samples were analyzed for BaP by isocratic reverse-phase HPLC with an octadecylsilane (C18) column (4.5 x 50 mm precolumn with 4.5 x 250 mm column) and methanol as the mobile phase. The flow rate was 0.7 ml/min and the eluent was passed through UV-VIS (ultraviolet visable; Beckman  reconstituted toluene, ethyl acetate, and methanol fractions were analyzed for BaP metabolites using a modification of the gradient system described by Salhab et al. (24). The column and detectors used were as for the isocratic separation, but the column was preequilibrated with starting mobile phase, 55% methanol:45% water, for at least 30 min before sample injection. After sample injection, the mobile phase was held at 55% methanol for 1 min. The amount of methanol was then increased by linear gradient to 86.5% MeOH over 30 min, held at 86.5% MeOH for 14 min, increased to 100% MeOH over 2 min, and held at 100% MeOH for 24 min. The column was then returned to the starting conditions. The retention times of BaP metabolite standards used in this system have been published elsewhere (20) except for BaP-3-, 7-, and 9-glucuronides, which eluted at 5.4, 5.8, and 5.6 min, respectively. Samples of dried methanol extracts and of the aqueous phase were incubated overnight at room temperature with Iglucuronidase or sulfatase, as described previously (25).
Statistical comparisons were performed with a 2-factor analysis of variance. To model the simultaneous effects of pretreatment and dose, statistical analyses of the experimental data were performed using the SAS (26) general linear models procedure. Pretreatment and dose level were modeled as separate main effects. A cross-products term was induded to assess potential effect modification (interaction). In no instance did the interaction term have a significant impact on comparison of the main effects; therefore, the reported analyses are of the main effects only. Outcome variables were the concentration of metabolites in blood and mucosa, the total metabolites found in postinfusate, and the postinfusate fluid volume. Where appropriate, a Student's t-test was used for other comparisons.

Results
Low monooxygenase activity was evident in intestinal microsomes from control catfish. HPLC analysis of the BaP metabolites formed from microsomal incubations   showed that the major metabolites were 3-OH-, 7-OH-, and 9-OH-BaP, BaP-diones, BaP-7,8-dihydrodiol (BaP-7,8-D), and BaP-9, 10-dihydrodiol (BaP-9, 10-D) ( Table  2). 3-OH-BaP accounted for 25-35% of the primary BaP metabolites formed by intestinal microsomes. The apparent Km for BaP (AHH) in intestinal microsomes from fish fed vehicle-treated chow alone was 1.83 ± 1.06 gM. Intestinal microsomes from catfish treated with BNF demonstrated a significant 5.6-fold increase in the AHH V value ( Table 3). The intestinal microsomes from BNF-treated catfish also had a 6.2fold higher EROD activity (  were used for dosage considerations in the in situ intestinal preparations. Total BaP Meq entering the systemic circulation in the in situ intestinal preparation varied with dose and with BNF treatment of the fish. A 10-fold increase in BaP dose administered resulted in a significant 3.0-6.3-fold increase in systemically available (blood) BaP Meq (Fig. 2). BNF pretreatment resulted in significant 5.5and 2.6-fold increases in systemically available BaP Meq for the 2 and 20 IM doses, respectively (Fig.  2). Analysis of radioactivity entering the systemic circulation for each of the in situ treatments indicated that the increase in BaP  Table 4). The in situ oxidative profile was similar to those demonstrated in in vitro studies, with the exception that hydroxylated metabolites were quantitatively much less important. Conjugates that predictably represented a significant fraction in situ consisted primarily of glutathione, sulfate, and glucuronide conjugates. The percentage of total recovered radioactivity as metabolites in the in situ preps ranged between 8.3 and 17.3% for blood and 5.3 and 10.2% for the mucosa. For all treatments the mucosa contained much higher absolute BaP and metabolite concentrations than blood (Tables 4 and 5). With the exception of BaP diones at the mucosal 20 jiM dose and hydroxy BaP at the blood 20 pM dose, BNF treatment resulted in greater concentrations of metabolites in both the intestinal mucosa and the perfusing blood. This increase was significant for six of the nine reported metabolite classifications in blood and for two of nine in mucosa. When metabolite concentrations were ranked based on their relative abundance among the major metabolites reported, several patterns emerge (greatest abundance = highest rank). Conjugate concentrations were consistently the highest ranked category in both blood and mucosa in both control and BNF-treated animals. BaP diones as a group were the second highest category for all treatments in the blood and the controls at both concentrations for the mucosa. Interestingly, the relative amounts of diones Environmental Health Perspectives * Volume 106, Number 3, March 1998 dropped precipitously relative to those of other metabolites in the BNF treatments for both concentrations in mucosa. In terms of ranking among metabolites, relatively more OH-BaP was present in the mucosa than in the blood.
The total BaP Meq, metabolite abundance, and postinfusate volumes recovered from the intestinal lumen following the 1hr in situ exposure are shown in Table 6. Postinfusate volumes recovered were significantly lower with BNF treatment at both the 2 and 20 pM BaP dosages. Average total BaP Meq concentrations in the recovered postinfusate were 744, 1,265, 9,791, and 8,484 pmol for the 2 pM control, 2 pM BNF-treated, 20 pM control, and 20 pM BNF-treated groups, respectively. When the BaP Meq levels were examined on a per-unit basis, the BNF groups consistently demonstrated higher values. BaP Meq of postinfusate, mucosa, and blood on per-unit bases indicate that within a treatment, the BaP Meq of mucosa was 1,855, 667, 1,404, and 546 times higher than that of the postinfusate for the 2 pM control, 2 pM BNF, 20 pM control, and 20 pM BNF treatments, respectively. Similarly, the BaP Meq of mucosa was 20,622, 6,620, 26,427, and 11,902 times higher than that of the blood for the same treatments. For both the mucosa-postinfusate and mucosa-blood comparisons, substantial reductions in the concentration differential within a dose treatment were evident with BNF treatment. Metabolites comprised 12.9, 9.4, 9.5, and 9.0% of the total radioactivity in the postinfusate for the 2 pM control, 2 pM BNF, 20 pM control, and 20 pM BNF treatments, respectively. BNF treatments resulted in elevated average metabolite concentrations for seven metabolite classifications at 2 pM and four metabolite classifications at 20 pM.
The metabolite profiles of radioactivity in postperfusate blood and the intestinal mucosa following [3H]-BaP exposure via infused blood are shown in Table 7. BaP and a wide variety of metabolites were evident in both the blood and mucosa. The major constituent for both the blood and mucosa was the parent BaP. BNF increased the total metabolites twofold in the blood and 1.8-fold in the mucosa; however, total BaP Meq (including BaP) concentrations were not significantly different between treatments. Significantly greater amounts of OH-BaP, BaP-diones, BaP-7,8-D, and BaP-9,10-D were evident in the blood and BaP-7,8-D in the mucosa upon induction than in controls. On an equivalent unit basis, the mucosa had three orders of magnitude higher BaP Meq concentrations than the postinfusate blood. After the BaP parent, the next largest categories in the blood were BaP diones, conjugates, unidentified metabolites, and OH-BaP, respectively, for both control and BNF treatments. The mucosa demonstrated a somewhat different profile from the blood, with the BaP-diones much less prevalent and OH-BaP, BaP-9,10-D, and conjugates more prevalent than the other metabolites.
6-Methyl-BaP, identified as a potentially hazardous BaP metabolite in mammalian systems, was found in blood, mucosa, and postinfusate of the catfish in situ preparation bStatistical comparisons were performed with 2-factor analysis of variance; significant at p<0.05.
cThe unidentified fraction was radioactivity not eluted from the Cl, matrix and is likely to include break-down products from glutathione and glucuronide conjugates of BaP metabolites (see text).  (Tables 4-7). Compared to other reported metabolites, 6-methyl-BaP was found in small quantities in the blood and mucosa and proportionally larger amounts in the postinfusate. BNF pretreatment did provide a significant increase in 6-methyl-BaP for those fish exposed through the blood (Table 7). Generally, more 6-methyl-BaP was evident with increasing dose for the mucosa and postinfusate.

Discussion
Intestinal CYPIA activity has been examined in several fish species under control and induced conditions. Control AHH activities of intestinal microsomes from vendace, perch, roach (27), scup (28), toadfish (15), and spot (29) (29,31). Toadfish administered BaP in the diet (10 mg/kg food at 5% body weight every third day) experienced a 9.7-fold increase in AHH activity (15). AHH activities of induced animals in these studies ranged from 320 to 720 pmol/min/mg protein (15,29,31). Similarly, induced EROD activities were 36and 10-fold higher for spot exposed to 3-MC (29) and mummichog exposed to BNF (BNF 250 mg/kg food) (30), with activities ranging from 667 to 2,018 pmol/min/mg protein. BNF administration in the present study resulted in an increase in AHH activity from 12.5 to 70.2 pmol/min/mg protein and EROD activity from 1.86 to 11.5 pmol/min/mg. CYPIA 'The total volume left in the intestine after the perfusion differed significantly between control and BNF treatment groups but was not dependent on initial BaP concentration; initially, 4 ml was infused into each intestinal preparation. bStatistical comparisons were performed with 2-factor analysis of variance; significant at p<O.05. Intestinal microsomes from catfish maintained on the control diet produced several major metabolites, including 3-OH-BaP, other benzo-ring phenols, and a variety of dihydrodiols. This group of metabolites was similar to those produced in the liver of other fish species such as sheepshead minnow, killifish (32), starry flounder, English sole (33), and scup (34).
Intestinal microsomes of control catfish demonstrated a 18.7-fold lower total BaP metabolite yield than that reported for the liver (16). The percentages of individual metabolites, however, were quite similar for 3-OH-BaP (intestine, 38%; liver, 38.5%), 7-OH and 9-OH BaP (intestine, 8.4%; liver, 1 1.1%), and BaP-7,8-D (intestine, 6.9%; liver, 11.7%). Substantial differences were observed for the diones (intestine 25.4%; liver 10.5%). BaP-7,8-D, a precursor to the major putative carcinogen, was formed to a significantly greater degree as in other fish species and in liver microsomes than by their mammalian counterparts (35-37). Although large quantitative differences exist for total BaP metabolite production between hepatic and intestinal microsomes of controls, induction studies utilizing BNF under identical exposure conditions as used presently have demonstrated nearly identical AHH activities for the two organs (16). The importance of the intestine relative to the liver in biotransformation of dietary BaP may be linked to the level of dietary induction of the intestine.
Within individual treatments of the in situ studies, mucosal BaP Meq concentrations were 546-1,855 times higher than those for the postinfusate micelle solution. Similarly, mucosal BaP Meq concentrations were 6,620-26,427 times higher than the blood. The differences for mucosal-blood comparisons were greatest for control treatments at either the 2 or 20 IpM dosage regimes (mucosa was 20,622-26,427-fold higher than blood). BaP Meq concentrations in the mucosa, postinfusate, and blood all increased with BNF preexposure. The relative increases, however, were much larger for the blood and postinfusate than for the mucosa. Effectively in face of absolute increases, BNF pretreatment lowered mucosal BaP Meq concentrations relative to either the intestinal lumen or the blood. These findings may be related to several events coinciding with BNF preexposure: 1) an increase in metabolite formation; 2) an apparent reduction in the recoverable micelle volume in the intestinal lumen over the duration of the in situ perfusion; and 3) a relatively greater bioavailability of BaP Meq to the systemic circulation.
BNF, in many fish species, is known to be an effective inducer of CYPIA activity (38-40) as well as a modest inducer of phase 2 activities such as glucuronosyl transferase (41) and glutathione-S-transferase (16,30). Metabolism may act upon intestinal bioavailability by providing substrates for specific transporters such as the multispecific organic anion transporter (42,43) or by metabolizing the lipophiic BaP parent to a metabolite with a polarity more favorably suited for absorption. Previous studies in which 3-OH-BaP was administered into the intestinal lumen of the catfish have shown that primarily the conjugates of 3-OH-BaP were transported from the mucosa to the blood (44). Similarly, sulfate and glucuronide conjugates of 9-OH-BaP have been shown to be readily absorbed intact from the intestinal lumen into the systemic circulation of the catfish (44). Given the similarity in lipid solubility of 3-OH-BaP and BaP (compared to that in conjugates) and what perhaps may be a ready transport of conjugates, increased metabolism may facilitate movement of lipophilic BaP Meq from the lumen to the circulation. Although the systemic availability of BaP Meq increased 2.6-5.5-fold with BNF pretreatment, the increase in metabolites available to the blood represented only 10.2-23.1% (depending on dose) of the increased Meq entering the systemic circulation. This information suggests that although metabolism was likely to have an effect, it probably is not the sole determining factor in the changes in bioavailability.
Perhaps BNF exposure alters cellular structure and/or integrity thereby affecting bioavailabiity. BNF has been shown to elicit structural and biochemical changes in fish (45,46) as well as to inhibit metabolism (phase 1 and 2) (16,4X. Brown bullheads exposed to BNF at high concentrations (500 mg/kg diet) in the diet exhibited reduced body weights, physical deformities, and epithelial hyperplasia on body surfaces. Similar effects such as reduced body weights and gill and fin lesions have been observed with other Ah receptor agonists (TCDD, for example) in black bullheads (48). On a molecular basis, BNF (100 mg/kg) has been shown to alter hepatic phospholipid metabolism in the rainbow trout, with a 34% increase in microsomal phospholipid con, tent within 24 hr of BNF administration (46). The BNF dosages used in the current study were 50 times lower than those exhibiting overt toxicity (45), 333 times lower than doses used in lipid studies (46), and much lower than those commonly used in hepatic induction studies (49). Although histology was not performed and signs of gross toxicity were not evident in in situ prepared fish, the selective reduction in perfusate volumes with dietary BNF pretreatment indicates that the catfish gastrointestinal tract was different in some manner because of BNF administration. Reduction in postinfusate volumes over the duration of the perfusion by an unknown mechanism may have increased the BaP concentration gradient from the intestinal lumen to the systemic circulation. This increase in the concentration gradient, a solvent drag phenomenon, or a permeability change may have increased the net influx of BaP Meq.
A third possible explanation for the increase in BaP Meq bioavailability with BNF exposure may relate to the induction of transporter function. Although a specific transporter has not been identified as being a factor in these studies, it is known that BNF induces the function of at least one transporter in the intestine of catfish (50). This transporter, P-glycoprotein, is known to transport BaP in mammalian liver cells (51). It is not known if metabolites of BaP are similarly transported.
When in situ intestinal study comparisons are made between metabolism of catfish in the current study and toadfish fed BaP (a weaker inducer than BNF) at 10 mg/kg food at 5% of body weight every 3 days, we find that approximately 8.3-17.3% of BaP in the blood was metabolized in the catfish preparation compared to 62-90% for the toadfish (15). In vitro AHH activities for pretreated control and induced toadfish had values of33 and 320 pmol/min/mg microsomal protein, respectively. These values are nearly threefold higher than controls and 4.6-fold higher than induced activities, as demonstrated for catfish in the current study. Such apparent differences in levels of biotransformation may account for the large differences in amounts of metabolites produced in the in situ intestinal preparation between the two studies. In addition to enzymatic activities, several experimental differences may contribute to the contrasting in situ studies. These differences include species (catfish vs. toadfish), species source (hatchery vs. field), inducer selection (BNF vs. BaP), length of perfused intestinal segment (isolated segment vs. whole intestine), circulatory perfusion method (dosed vs. open), BaP carrier vehicle (micelle vs. oil), and the method of metabolite analysis (HPLC vs. differential extraction). In vivo studies with rats (52) and fish (53) also indicate extensive metabolism of dietary BaP by the intestine. Further study is necessary to determine if differences are associated with the species or the experimental protocols.
In the in situ preparations, high concentrations of BaP-7,8 and 9,1 0-D were found in the intestinal mucosa relative to those in the blood and micelle postinfusate. These dihydrodiols appear to arise from the relatively robust activity of catfish mucosal epoxide hydrolase on the respective BaPoxides (16). It is likely that the higher BaP-7,8 and 9,1 0-D concentrations present in the intestinal mucosa are primarily a result of buildup at the site of production, as orally administered BaP-7,8-D has been shown to be readily transferred from the fish intestine (54). Quantitatively, the proportions and absolute concentrations of BaP-7,8 and 9,10-D were greater for BNF-pretreated animals. BNF  Proportional increases in the dihydrodiol contribution with induction have been demonstrated in a variety of mammalian studies and are due to induction of epoxide hydrolase as well as CYP1A (56). In the catfish intestine the elevated dihydrodiol concentrations with BNF pretreatment appear to be due to increased CYPIA activities in face of high but noninduced levels of epoxide hydrolase activity (16). Importantly, the catfish intestine responds to dietary BNF by producing greater proportions of potentially hazardous BaP metabolites that may be transported by the systemic circulation to distant sites. Classic toxicokinetic studies with intravenous BaP and BaP-7,8-D in the winter flounder indicate higher volumes of distribution (Vd) and clearance rates with BaP-7,8-D (54). Clearly these features offer contrasting risks because the increased polarity of BaP-7,8-D facilitates elimination, whereas a larger volume of distribution poses greater access of a more proximate carcinogen (BaP-7,8-D) to susceptable macromolecules.
6-Methyl-BaP and 6-OH-methyl-BaP (data not included) were shown to be formed in the catfish in situ intestinal preparation. To the authors' knowledge this is the first time these metabolites have been tentatively identified in a fish species. 6-Methyl-BaP has been demonstrated in mammals to arise in vivo from the methylation of BaP by methyl transferase (57), whereas 6-OHmethyl-BaP results from a P-450-mediated hydroxylation of the methylated metabolite. 6-Methyl-BaP and 6-OH-methyl-BaP as well as the sulfate, phosphate, and acetate esters of 6-OH-methyl-BaP, when given to animals, have been shown to form protein and DNA adducts through the 6-methylene group (58). These adducts may arise from an SN2 (substitution nucleophilic biomolecular) reaction of the ester of 6-OH-methyl-BaP with cellular nucleophiles or by the sulfation of 6-OH-methyl-BaP and loss of the sulfate anion possibly to form a reactive carbocation (58,59). Further investigation will be necessary before the importance of these potential pathways of BaP activation are known for the fish intestine.
Diones were major contributors to the total metabolites in the in situ intestinal preparation as they were for the microsomal positional metabolism. Intestinal mucosa contained much higher concentrations of diones on a per-unit basis than either the blood or postinfusate. In general, the amount of diones increased from the 2 1M to the 20 pM dose for both control and BNF comparisons. BNF pretreatment resulted in increased dione concentrations for both the 2 IM and 20 pM concentrations of the blood and the 2 pM concentration in the mucosa. For the 20 pM treatment, dione concentrations in mucosa demonstrated a large drop with BNF pretreatment. Diones constituted a lower percentage of the total metabolites for BNF treatments than in controls for mucosa and marginally lower in the blood. This response is in contrast to the relative increases in percentages of BaP-7,8 and BaP 9,10-D on BNF pretreatment. A likely explanation for these findings is that induction of CYPIA by BNF favors formation of benzo-ring arene oxides, the precursors to benzo-ring dihydrodiols.
When BaP was administered into the intestinal lumen of the in situ preparations, between 33.9 and 60.1% (depending on treatment) of the metabolites in the postinfusate were diones. This compares to 7.3-32.4% for the mucosa and 16.0-31.4% for the blood across identical treatments. For studies where BaP was administered through the blood, diones accounted for 49.6 and 49.0% of the blood metabolites for the 2 pM control and BNF treatments, respectively. The mucosa in these same treatments contained between 6.9 and 7.5% of total metabolites as diones. Although the mucosa contained the highest absolute dione content, it also accounted for the greatest BaP Meq concentrations and total net metabolism. Conversely, the postinfusate and blood, although not producing metabolites to the same degree as mucosa, were represented to a much greater degree by dione formation. There are interesting corollaries of these observations to the situation in many invertebrates in which P450 metabolism is low and dione formation is of greater importance (60). Although comparisons with intestinal or in situ preparations are not available, the percent of metabolites as diones has been reported for hepatic microsomes from a variety of fish species (6). Of the studies examined, the percent of diones formed by fish ranged from 3.8 to 28%, with a median value of approximately 13%. The percent of metabolites as diones reported here for the in situ intestinal preparation generally fell into this range except for the high values for the postinfusate across all treatments and the postperfusate blood (control and BNF pretreated) of the blood exposure studies. Large-scale air oxidation of the BaP appears to be an unlikely explanation for the high levels of diones in these samples because preinfusate handled in an identical fashion but without exposure to tissues did not exhibit significant dione production. Pathways of xenobiotic oxidation that characteristically form BaP diones have been identified with the vasculature and hematin of mammals (61). Dione formation in mammals is thought to occur by the intermediacy of a BaP cation radical (62) and 6-OH-BaP (63,64) through a one-electron oxidation mechanism. This oxidation may occur with BaP acting as a reducing cosubstrate for the oxidation of arachidonic acid by prostaglandin H synthase (PHS) or by reactions catalyzed by heme containing proteins and lipid hydroperoxides. Tissues with low monooxygenase activity and high PHS concentrations such as the alimentary tract and vasculature are favorable sites for this oxidation route (61). Concentrations of PHS in fish tissues are unknown; however, P450 activities generally are lower in the vascular (65-67) and intestinal (16) compartments than in the liver, especially in uninduced animals. Predictably, an attempt with liver microsomes to detect the 6-oxy-BaP free radical in fish was largely unsuccessful (6). Non-P450-dependent metabolic routes and transport differences in the intestine and the vasculature are plausible explanations for the prominent role of diones in these select studies and samples.
Conjugates represented a major component in the blood and intestinal mucosa, accounting for between 26.5 and 65.0% and 31.4 and 51.3% of the recoverable metabolites, respectively. Blood and mucosa of controls demonstrated greater composite conjugate concentrations than the unconjugated metabolites at the 2 pM dose, whereas at the 20 pM dose the unconjugated metabolites attained 1.9-2.0-fold higher concentrations. BNF treatment, while increasing absolute concentrations of all metabolites, appeared to negate these findings, as the unconjugated metabolites predominated at both the 2 and 20 pM concentrations. Both dose and BNF pretreatment appeared to facilitate in absolute terms the increased production of intestinally derived metabolites. Conjugate concentrations, although sensitive to these mechanisms, demonstrated incongruencies with the larger response of the unconjugated metabolites. Relative limitations in phase 2 metabolism in face of increased concentrations of phase 1 metabolites may account for the observed findings. This concept is supported by previous BNF induction studies with catfish intestine that have demonstrated little induction of glutathione-Stransferase and no induction of UGT or ST (16). In addition, BNF treatment also increases CYP1A production of BaP-7,8oxide and BaP-9,10-oxide, which in turn leads to increased BaP-7,8-D and 9,10-D formation, as well as 7-and 9-hydroxy BaP (Fig. 3). The resulting BaP-dihydrodiols are poorer substrates for glucuronidation than BaP-phenols (68), which leads to a buildup of unconjugated dihydrodiols relative to hydroxy-BaP. Strict   KmIVmaX as well as availability considerations. Intestinal mucosal homogenates from flounder administered dietary BNF when incubated with BaP at 0.5 and 5.0 pM exhibited greater amounts of BaP conjugates, whereas at 50 and 250 pM, conjugates fell relative to the polar metabolites and unmetabolized BaP (17). A similar dose dependence appears to exist here for the in situ intestinal metabolism of BaP.
The water-soluble fractions and HPLC peaks eluting before 10 min in the present study are likely to include a mixture of sulfate, glucuronide, and glutathione conjugates of the oxidative metabolites of BaP (Fig. 4). The large number of potential conjugates from BaP-phenols, BaP-dihydrodiols, and BaP-oxides, in light of their overlapping physicochemical properties, made isolation of individual polar conjugates difficult based on retention characteristics. Incubation of radioactivity eluted from the C18 matrix beads by water and methanol with 1-glucuronidase or sulfatase suggested that up to 20% of the conjugates found were a mixture of glucuronides and sulfates. More than 80% of the conjugates were not hydrolyzed by sulfatase or P-glucuronidase, suggesting that these were glutathione conjugates and further metabolites of glutathione conjugates. Others have shown that glutathione conjugates were the major metabolites of orally administered BaP (0.1-2 mg/kg) excreted in vivo in bile of several fish species (6,69). In addition to the water and methanol fractions eluted from the C18 matrix beads, there is evidence that a portion of the unidentified radioactivity not eluted from the C18 beads included breakdown products of glucuronide and glutathione conjugates [ Table 1; Tong and James, unpublished observations; (70)].
Intestinal microflora are thought to be minimal contributors to the observed findings. There is no evidence that these organisms contain the P450s or conjugative enzymes involved in BaP oxidation or conjugation [ Fig. 4; (71-73)]. Microflora, however, do contain reductive and hydrolytic enzymes. Degradative reactions such as dehydroxylation and hydrolysis of glucuronides may decrease postinfusate metabolite concentrations. This effect is thought to be minimized because fasting as well as dearing fecal material would be expected to reduce bacterial numbers and their metabolic contribution (74).
A considerable degree of variation was evident in all aspects of these studies. Fish are inherently variable relative to a number of key biotransformation enzymes (75). Intestinal studies pose other challenges. Catfish because of their poikilothermic nature and feeding behavior show variations in food consumption and hence in in vivo intestinal induction. This is problematic because healthwise they do not tolerate long-term repetitive handling as in gavage feeding. In addition, variable boundaries imposed by the circulation in perfusion studies, the somewhat variable length of the perfusion segment because of the state of relaxation and contraction of the in situ intestine, the wide scope of available biotransformation pathways, and the dynamic nature (turnover) of the mucosal cells containing uptake and biotransformational sites all contribute to variability.
In summary, the systemic bioavailability of BaP molar equivalents from the intestine was significantly greater with higher BaP dosages and BNF pretreatment. BNF generally increased metabolite production; however, increases in bioavailability could not be accounted for solely by changes in metabolism. Intestinal formation and systemic uptake of potentially hazardous metabolites and detoxification products of BaP in the catfish intestine appear to be related to dose and BNF pretreatment through an interplay of primary and secondary biotransformation pathways. Conjugates were proportionally favored under low-dose uninduced conditions, whereas benzo-ring diols were proportionally more important upon BNF preexposure. Clearly the interplay of dose, exogenous agents, and intestinal function are important factors in the uptake, disposition, and risk associated with dietary BaP.