Metabolism of Vitamin A and Its Active Metabolite All-trans-retinoic Acid in Small Intestinal Enterocytes

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Vol. 295, Issue 3, 979-985, December 2000

**Metabolism of Vitamin A and Its Active Metabolite All-trans-retinoic Acid in Small Intestinal Enterocytes¹**

Alfonso Lampen, Silke Meyer, Thomas Arnhold² and Heinz Nau

Zentrumsabteilung für Lebensmitteltoxikologie, Tierärztliche Hochschule Hannover, Hannover, Germany

	Abstract

Top Abstract Introduction Experimental Procedures Results Discussion References

Retinol and its metabolites (retinoids) are essential for growth and cell differentiation, particularly of epithelial tissue.Retinoids mediate most of their function via interaction withretinoid receptors (retinoic acid receptors and retinoid X receptors),which act as ligand-activated transcription factors controllingthe expression of a number of target genes. We have investigatedwhether retinoid receptor ligands such as all-trans-retinoic acid(RA) are formed in the human intestinal epithelium from dietaryvitamin A. We show here that retinol was metabolized to its activemetabolite, all-trans-RA, by isolated cytosolic fractions of humansmall intestinal enterocytes and by human Caco-2 cells. All-trans-RAwas metabolized by human small intestinal microsomes to at leasttwo metabolites (all-trans-4-hydroxy-RA and all-trans-4-oxo-RA).When Caco-2 cells were incubated with all-trans-RA, at least threemajor polar metabolites (all-trans-4-hydroxy-RA, all-trans-4-oxo-RA,and 13-cis-4-hydroxy-RA) were identified by HPLC-UV. The cytochromeP450 (CYP) 1A1 inhibitor $alpha$ -naphthoflavone inhibited the metabolismof all-trans-RA, whereas the CYP1A1 inducer $beta$ -naphthoflavone inducedthe metabolism of all-trans-RA, suggesting that CYP1A1 is involved.The induction of CYP3A by rifampicin enhanced the metabolism,and the induction of all-trans-RA metabolism was also observedafter preincubation of the cells with all-trans-RA. Liarozolealmost completely inhibited the RA metabolism. The specific retinoicacid metabolizing CYP26 was induced after RA treatment in Caco-2cells. It is concluded that in addition to CYP1A1 and CYP3A, CYP26may be the main CYP enzyme responsible for the metabolism of all-trans-RAin enterocytes. Active ligands such as all-trans-RA are formedin intestinal epithelialcells.

	Introduction

Top Abstract Introduction Experimental Procedures Results Discussion References

Retinol (vitamin A) and its metabolites (retinoids) are essential for growth and cell differentiation, particularly of epithelialtissue (for review, see Nau and Blaner, 1999). Although smallintestinal enterocytes play a central role in the absorption andmetabolism of dietary retinol, very little is known about thefunction of retinoids in the gastrointestinal epithelium and themolecular basis of retinoid metabolism in the human intestine.Retinyl esters are enzymatically converted to retinol in the intestinallumen before absorption, and carotenoids are converted to retinolin enterocytes (Blomhoff et al., 1990). Inside the enterocyteretinol is bound to CRBPII, followed by re-esterification to retinylesters by the lecithin-retinol acyl transferase (LRAT) or acyl-CoA:retinol-acyltransferase(ARAT). Together with phospholipids, cholesterol, and triglycerides,the retinyl esters are packed into chylomicrons and released intothe lymph. Retinol can either be stored in the liver, primarilyas retinyl esters, or be secreted into plasma bound to its specifictransport protein, retinol-binding protein (Ong, 1993). To date,it is not known whether retinol is oxidized intracellularly bythe human small intestinalenterocyte.

To understand the physiological roles of retinoids in the enterocyte, it is crucial to know whether retinoic acid (RA) orother active metabolites are formed in the small intestinal enterocytesfrom dietary vitamin A and how RA may be further metabolized inthe human enterocytes. Such knowledge is also clinically importantbecause RA has been used in the treatment of certain human diseasessuch as acute promyelocytic leukemia. Still, unsolved problemsare the limited bioavailability of RA (50%) and the rapidly developingRA resistance in therapy of acute promyelocytic leukemia. Intestinalmetabolism of RA may contribute to these effects (Regazzi et al.,1997).

Cytochrome P450 (CYP) 3A enzymes account for 70% of the total concentration of CYP enzymes in the small intestine. It hasbeen hypothesized that metabolism mediated by CYP enzymes in thesmall intestine may, at least in part, be responsible for thelow and variable oral bioavailability of most drugs that are substratesof these enzymes (Lampen et al., 1995). It is well known thatCYP enzymes are involved in the metabolism of all-trans-RA. Usingrat liver microsomes it has been shown that CYP3A as well as CYP2C8is capable of metabolizing all-trans-RA to 4-hydroxy metabolites(Martini and Murray, 1993; Nadin and Murray, 1999). However, itis not known which CYP enzymes are involved in a potential intestinalmetabolism of RA. Recently a newly RA-specific CYP enzyme calledCYP26 (CYPRAI) that metabolizes RA to 4-hydroxy-, 4-oxo-, and18-hydroxy-RA was cloned (Fujii et al., 1997; Ray et al., 1997).This enzyme has been detected in adult human liver and brain andin mouse embryo as early as embryonic day 8.5 in specific regions(Ray et al., 1997). To the best of our knowledge, this RA-specificenzyme has not been detected in the human intestine and consequentlyits impact on retinoid metabolism and regulation in the intestineis notknown.

Most effects of vitamin A are attributable to its active metabolites; all-trans-RA, 9-cis-RA, and all-trans-4-oxo-RA are knownto be biologically active. The active forms of RA exert theireffects by serving as ligands for nuclear receptors called RARs(Petkovich et al., 1987) and RXRs (Mangelsdorf et al., 1992),which act as ligand-activated transcription factors controllingthe expression of a number of target genes. In the presence ofRA, an RAR-RXR heterodimer is able to regulate expression of aset of genes (Chambon, 1996). All-trans-RA acts as a ligand forthe RAR and therefore represents a biologically active form ofvitamin A. We hypothesized that biologically active retinoidsmay be formed in the gastrointestinal tract and may act as retinoid-receptorligands controlling various processes in the intestinal mucosa.We also hypothesized that all-trans-RA may be metabolized in theenterocyte to more polar metabolites and that CYP enzymes maycontribute to thismetabolism.

	Experimental Procedures

Top Abstract Introduction Experimental Procedures Results Discussion References

Materials and Reagents. All-trans-retinol and all-trans-RA were purchased from Sigma (Deisenhofen, Germany) and 13-cis-4-oxo- and all-trans-4-oxo-RAwere kindly provided by Hoffmann-La Roche (Basel, Switzerland).Lyophilized analytical grade BSA was purchased from Sigma (St.Louis, MO). Isocitric acid, NADP, and isocitrate dehydrogenasecame from Boehringer Mannheim (Mannheim, Germany). All other chemicalswere purchased from Merck (Darmstadt, Germany) or Sigma in thehighest available purity. Water for HPLC was purified using aMilli-Q water purification system (Millipore, Eschborn, Germany).Liarozole was a generous gift from Janssen Research Foundation(Beerse, Belgium). Stock solutions of retinoids were preparedin ethanol (or dimethyl sulfoxide) at a theoretical concentrationof 0.1 mg/ml, which were subsequently photometrically corrected.These solutions were kept in glassware at $-$ 20°C. All laboratorymanipulations involving the retinoids (preparation of dosing solutions,drug treatment of cells, collection of samples, and analyticalprocedures) were performed in dark rooms under dim yellow lightto prevent photoisomerization. The Caco-2-TC7 cell line (TC7)was a generous gift from Dr. Alain Zweibaum (Institut Nationalde la Santé et de la Recherche Médicale U178, Villejuif Cedex,France).

Cell Culture. Caco-2 and Caco-2-TC7 cells were kept in Dulbecco's modified Eagle's medium supplemented with 10% fetal calf serum (Boehringer,Ingelheim, Germany) at 37°C in a humidified atmosphere of 5% CO₂-air.

Retinoid Analyses. Retinoids in supernatants and cells were analyzed using a reversed-phase HPLC method with gradient elution after sample enrichmentwith liquid-liquid and solid-phase extraction (Collins et al.,1992). According to this method, samples were extracted with isopropanol,and the supernatants were then extracted on solid-phase extractioncartridges before introduction into the HPLC system. Further processingwas performed as described previously by Collins et al. (1992).UV detection of the HPLC eluate was performed at 340 and 356 nmby use of a two-channel SPD-10AV detector (Shimadzu, Duisburg,Germany).

Recovery and reproducibility of the assay and calibration with an external method were reported previously (Collins et al.,1992

). Identification of HPLC peaks was based on comigration withauthentic retinoids and on coincidence of the absorbance ratios(i.e., ratio of peak areas) at the two wavelengths of detectionwith that of the standardretinoids.

Preparation of Cytosolic and Microsomal Fraction of Human Intestinal Enterocytes. Human small intestinal samples for the isolation of cytosol and microsomes were obtained from the Klinik für Abdominal undTransplantationschirurgie (Medizinische Hochschule Hannover, Hannover,Germany), and the collection of human small intestinal samplesfor research was approved by the Ethical Committee of the MedizinischeHochschuleHannover.

Human enterocytes were isolated according to the method described by Pinkus (1981)

. Cytosolic fractions and microsomes wereisolated using a differential centrifugation procedure describedby Guengerich (1982)

with the modifications that a 0.1 M phosphatebuffer (pH 7.4) be used instead of a Tris buffer and that theultracentrifugation steps (100,000g) be reduced to 45 min. Cytosolwas prepared by centrifuging the supernant obtained from the secondspin at 105,000g for 1 h. Protein concentrations were measuredusing the bicinchoninic acid method (Smith et al., 1985

) and aBSA standard curve. The protein concentrations of the microsomalsuspensions were adjusted with 0.1 M phosphate buffer (pH 7.4).

In Vitro Metabolism of All-trans-ROH and Sample Preparation. Cytosolic fractions of human enterocytes were incubated for 25 min at 37°C. The incubations contained 1 mg of protein, 2 mMNAD, 2 mM dithiothreitol, and all-trans-ROH (added in 5 µl ofethanol) at various concentrations and were brought to a finalvolume of 0.5 ml by adding 150 mM KCl or 20 mM HEPES,respectively.

In Vitro Metabolism of All-trans-RA and Sample Preparation. All-trans-RA (10 µM) in 10 µl of ethanol was added to 1 ml of small intestinal microsomes (1.5 g of protein/l). The reactionwas started by adding 0.5 ml of an NADPH-generating system consistingof 2 mM EDTA, 10 mM MgCl₂, 0.84 mM NADP, 18 mM isocitric acid,and 667 U/l of isocitrate dehydrogenase. The reaction mixturewas incubated for 30 min at 37°C under aerobic conditions. Thereaction was stopped by the addition of a 3-fold volume ofisopropanol.

Metabolism of All-trans-RA in Caco-2 Cells. Caco-2 cells were cultured for 18 to 21 days (maximum of differentiation). All-trans-RA (10 µM) was added to the fresh culturemedium and incubated for 6 h. A cell pellet and cell medium volumeof 150 µl were extracted with a 3-fold volume of isopropanol,followed by short centrifugation and solid-phase extraction (seeabove).

Chemical Inhibition of All-trans-RA Metabolism in Caco-2 Cells. $alpha$ -Naphthoflavone, a selective CYP1A1 inhibitor (Chang et al., 1994), and liarozole, a inhibitor of the human RA 4-hydroxylaseactivity (CYP26), were dissolved in dimethyl sulfoxide. Ketoconazole,a selective noncompetitive CYP3A inhibitor at low concentrations(Chang et al., 1994), was dissolved in ethanol. The inhibitorsolution (10 µl) was added to 20 ml of medium. The final concentrationsranged from 0 to 750 µM. The samples were preincubated with theinhibitor for 60 min to inactivate the CYP enzymes. Then the substrateall-trans-RA was added and after an incubation period of 3.5 hat 37°C, the reaction was stopped by the addition of isopropanol(seeabove).

Preparation of RNA. Total RNA was prepared from freshly isolated cells according to the method of Chomczynski and Sacchi (1987). RNA concentrationswere determined spectrally with a UV-visible spectrophotometer(Perkin-Elmer Life Sciences, Foster City, CA), and the integrityas well the concentrations of RNA was checked in an agarose testgel using an RNA-standard (Eurogenitic, Seraing,Belgium).

RT-PCR Analysis. RT-PCR was carried out using Superscript II reverse transcriptase (Life Technologies, Karlsruhe, Germany) and Taq-polymerase(Qiagen, Hilden, Germany). The samples were then heated for 3min at 94°C to terminate the reverse transcription reaction. ThePCR was performed on 1 µl of a 1:10 dilution in water of a preparedcDNA. Primers for human CYP26 were nt 87-111 for sense and nt343-368 for antisense (GenBank accession number AF005418).Primers for human CYP1A1 were nt 5762-5784 for sense and nt 6689-6709for antisense (GenBank accession number X02612). Primers forhuman CYP3A4 were nt 1349-1376 for sense and nt 1702-1731 forantisense (GenBank accession number J04449). Primers for humanCYP3A5 were nt 1236-1266 for sense and nt 1517-1546 for antisense(GenBank accession number NM00777). Primers for human $beta$ -actinwere nt 371-391 for sense and nt 800-820 for antisense (GenBankaccession number X00351). PCR was performed with 0.5 U of Taq-polymerase(Qiagen, Hilden, Germany) in an automatic DNA thermal cycler (MWG,Ebersberg, Germany) by adding 30 µl of a PCR master mixture containingPCR buffer, MgCl₂ (to a final concentration of 1 mM) and 20 pmolof each primer to the cDNA samples. Thirty cycles [1 min at 94°C,45 s at 60°C for CYP26 (57°C for CYP3A4 and CYP3A5), and 45 sat 72°C] followed by an additional 5 min at 72°C were used. EachPCR included an aliquot of the reaction mixture without cDNA asa negative control. All amplifications were carried out for 30cycles. Under these conditions, all cDNA amplifications were foundto produce single products within a linear range (data not shown).PCR products were judged to be of the size appropriate for amplificationof the specific cDNA by comparison with molecular weight standardsincluded on each gel and with amplified plasmid cDNA of each gene.Amplified cDNA products were separated by agarose electrophoresis.Gels were stained with ethidium bromide, photographed using acharge-coupled device camera of Gel Doc 1000 (Bio-Rad, München,Germany), stored, and densitometrically analyzed using MolecularAnalysis (Bio-Rad). We thank Prof. M. Petkovich (Queen's University,Kingston, Canada) for providing us with the CYP26cDNA.

Statistics. Values for concentrations and concentration ratios were expressed as mean ± S.D. ANOVA was used for the statistical comparisonof twomeans.

	Results

Top Abstract Introduction Experimental Procedures Results Discussion References

Formation of RA in Small Intestinal Cells. When the cytosolic fraction of human enterocytes was incubated with all-trans-ROH, the active RAR ligand all-trans-RA wasformed. The formation was concentration-dependent (Fig. 1A), theK_m and V_max values for the metabolism of all-trans-ROH to all-trans-RAwere 15.4 µmol/l and 2 pmol/min × mg of protein, respectively.The formation of all-trans-RA was inhibited by 4-methylpyrazole(Fig. 1B). 4-Methylpyrazole (10 mM) inhibited the formation ofall-trans-RA by 85%, suggesting the involvement of ADHs. Furthermore,citral inhibited the formation of all-trans-RA. Citral (50 µM)inhibited the formation of all-trans-RA by 75%.

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Fig. 1. A, metabolism of all-trans-retinol to all-trans-RA in the cytosolic fraction of human small intestinal enterocytes. Different concentrations of retinol were incubated for 25 min with 1 mg of cytosolic protein, stopped with isopropanol, and extracted and analyzed using HPLC. B, metabolism of all-trans-ROH to all-trans-RA is inhibited by 4-methylpyrazole in human small intestinal cytosol. All-trans-retinol (10 µM) was incubated with different concentrations of 4-methylpyrazole for 25 min with 1 mg of cytosolic protein, stopped with isopropanol, and extracted and analyzed using HPLC. All values represent mean ± S.D. (n = 4).

Metabolism of All-trans-RA with Human Supersomes. To evaluate which CYP enzymes are capable of metabolizing all-trans-RA, we incubated a supermix (Gentest, Frankfurt, Germany)containing CYP enzymes of human liver (CYP1A2, CYP2C8, CYP2C9,CYP2C19, CYP2D6, and CYP3A4) and single human CYP1A1, CYP3A4,CYP2C8, CYP2E1, and CYP2D6 supersomes with all-trans-RA and measuredthe metabolites byHPLC.

Using human supermix all-trans-RA was metabolized after a 30-min incubation to all-trans-4-oxo-RA (0.888 pmol/h × pmol ofP450) and all-trans-4-hydroxy-RA (45.51 pmol/h × pmol of P450).With human CYP supersomes all-trans-RA was metabolized mainlyto all-trans-4-hydroxy-RA. All-trans-RA was metabolized by CYP3A4supersomes exclusively to all-trans-4-hydroxy-RA (3.15 pmol/h× pmol of P450). CYP1A1 supersomes metabolized all-trans-RA toall-trans-4-oxo-RA (0.12 pmol/h × pmol of P450) and to all-trans-4-hydroxy-RA(3.0 pmol/h × pmol of P450). After incubation with human CYP2E1all-trans-4-hydroxy-RA (1.1 pmol/h × pmol of P450) was formed.After incubation of CYP2C8 supersomes all-trans-4-hydroxy-RA (2.66pmol/h × pmol of P450) was formed. No metabolism of all-trans-RAwas detectable using CYP2D6-supersomes. Again no metabolism wasdetectable after incubation of all-trans retinol with CYP supersomesorsupermix.

Metabolism of All-trans-RA by Human Small Intestinal Microsomes. To investigate the further metabolism of all-trans-RA human small intestinal microsomes were used. After incubation of all-trans-RAwith human small intestinal microsomes, two major metaboliteswere identified by HPLC: all-trans-4-hydroxy-RA and 4-oxo-RA (Fig.2A).

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Fig. 2. A, metabolism of all-trans-RA in human small intestinal microsomes. Human small intestinal microsomes were incubated with 0.5 ml of NADPH-generating system and 20 µmol/l all-trans-RA (see Experimental Procedures). Incubations were stopped with isopropanol, and samples were extracted and analyzed using HPLC. All values represent mean ± S.D. (n = 3). B, concentration-dependent metabolism of all-trans-RA in Caco-2 cells. Caco-2 cells (2 × 10⁷ cells) were incubated with various concentrations of all-trans-RA. Four representative chromatograms are shown. Incubations were stopped with isopropanol, and samples were extracted and analyzed using HPLC.

Metabolism of All-trans-ROH and All-trans-RA in Caco-2 Cells. To investigate the formation and the further metabolism of all-trans-RA in more detail, an in vitro model (Caco-2 cells) wasused. When all-trans-ROH (7.5 µM) was incubated with Caco-2 cells(2 × 10⁷ cells) for 24 h we measured the formation of 0.33 µM all-trans-RAby HPLC, indicating that the formation of the RAR ligand all-trans-RAalso occurs in human Caco-2cells.

When Caco-2 cells were incubated with different concentrations of all-trans-RA the polar metabolites all-trans-4-oxo-RA, all-trans-4-hydroxy-RA,and 13-cis-4-hydroxy-RA were mainly formed (Fig. 2B). The peakeluting after 13-cis-4-hydroxy-RA (Figs. 2B and 3) could be notidentified due to the lack of a reference substance for 18-hydroxy-RA,but may represent 18-hydroxy-RA. The isomerization metabolites13-cis-RA and 9-cis-RA were also formed. The metabolism dependedon the concentration of the substrate used (Fig. 2B) and was time-dependent.The K_m was calculated to be 8.3 µmol/l.

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Fig. 3. Metabolism of all-trans-RA in Caco-2 cells after pretreatment of the cells with the CYP1A1 inducer $beta$ -naphthoflavone. Caco-2 cells were pretreated with 50 µM $beta$ -naphthoflavone for 72 h and then incubated with 10 µM all-trans-RA for an additional 6 h. Metabolites were extracted and analyzed using HPLC. Typical chromatograms are shown.

Induction and Inhibition of All-trans-RA Metabolism in Caco-2 Cells. When the Caco-2 cells were treated with $beta$ -naphthoflavone, a specific inducer of CYP1A1, the metabolism of all-trans-RA topolar metabolites was induced (Fig. 3). Fifty micromolar $beta$ -naphthoflavoneinduced the metabolism to the metabolites all-trans-4-oxo-RA,all-trans-4-hydroxy-RA, and 13-cis-4-hydroxy-RA by the factorof 10. On the other hand, the specific CYP1A1 inhibitor $alpha$ -naphthoflavoneinhibited the metabolism of all-trans-RA to the polar metabolitesby 76%. These results indicate that CYP1A1 was capable of metabolizingall-trans-RA and suggest that if induced, CYP1A1 metabolizes all-trans-RAin intestinalcells.

Ketoconazole inhibited the metabolism of all-trans-RA to the polar metabolites almost completely but only when high concentrations(>50 µM) were used, suggesting a more unspecific CYP inhibition(data not shown). Other CYP inhibitors such as sulfaphenazole(CYP2C inhibitor) or disulfiram (CYP2E1 inhibitor) showed no effecton the metabolism (data not shown). To investigate the role ofCYP3A enzymes in the intestinal metabolism of all-trans-RA, weused the Caco-2 clone TC-7, which has a higher catalytic activityof CYP3A than do Caco-2 cells (Raeissi et al., 1999

). Pretreatmentof the TC-7 cells with rifampicin induced the formation of all-trans-4-hydroxy-RA(Fig. 4A) and induced CYP3A4 and CYP3A5 gene expression (Fig.4B), suggesting that CYP3A enzymes are involved, at least in part,in the metabolism of all-trans-RA.

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Fig. 4. A, induction of the intestinal RA metabolism by a CYP3A inducer. Caco-2-TC7 cells were pretreated with 10 µM rifampicin or vehicle (control) for 24 h, washed three times with PBS, and incubated with 10 µM all-trans-RA for an additional 3 h. Metabolites were extracted and analyzed using HPLC. Values represent mean ± S.D. (n = 3). *, significant difference (P < .001; ANOVA) compared with pretreatment without rifampicin. B, induction of CYP3A4 and CYP3A5 gene expression in Caco-2 TC7 cells by rifampicin measured using RT-PCR. CYP3A4, CYP3A5, and $beta$ -actin gene expression was measured under optimal conditions using RT-PCR after treatment of Caco-2-TC7 cells with 10 µM rifampicin or vehicle (control) for 24 h. C, untreated; RIF, rifampicin-treated, 10 µM; M, marker.

Pretreatment of the Caco-2 cells with all-trans-RA induced the metabolism of all-trans-RA to polar metabolites by a factorof 3, indicating an autoinduction (Fig. 5). Liarozole, an imidazolederivative, is a known inhibitor of RA 4-hydroxylase activity(Fujii et al., 1997

; Sonneveld et al., 1998

), which is associatedwith the inhibition of CYP26. Liarozole inhibited the metabolismof all-trans-RA to polar metabolites very efficiently (Fig. 6).Liarozole (50 µM) inhibited the metabolism of all three polarmetabolites >90%, indicating that CYP26 is mainly responsiblefor the intestinal metabolism.

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Fig. 5. Autoinduction of the intestinal retinoic acid metabolism by all-trans-RA. Caco-2 cells were pretreated with 1 µM all-trans-RA or vehicle (control) for 24 h, washed three times with PBS, and incubated with 10 µM all-trans-RA for an additional 3 h. Metabolites were extracted and analyzed using HPLC. Values represent mean ± S.D. (n = 3). *, significant difference (P < .001; ANOVA) compared with untreated cultures.

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Fig. 6. Inhibition of all-trans-RA metabolism in Caco-2 cells by liarozole. Caco-2 cells were incubated with 10 µM all-trans-RA with or without different concentrations of liarozole. Metabolites were extracted and analyzed using HPLC. All values represent mean ± S.D. (n = 4).

Gene Expression of CYP26 in Caco-2 Cells After RA Treatment. Untreated Caco-2 cells expressed only small amounts of CYP26, almost at the detection limit (Fig. 7). When Caco-2 cells weretreated with all-trans-RA, the expression of CYP26 increased specificallyand in a dose-dependent manner (Fig. 7). This concentration-dependentinduction correlates well with the concentration-dependent formationof polar metabolites after incubation of all-trans-RA with Caco-2cells (Fig. 2B). When Caco-2 cells were treated with retinol (10µM for 24 h), CYP26 gene expression was also induced (Fig. 8),most probably because of the formation of all-trans-RA from retinolin the cell.

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Fig. 7. CYP 26 gene expression in Caco-2 cells measured using RT-PCR. CYP 26 and $beta$ -actin gene expression was measured under optimal conditions using RT-PCR after treatment of Caco-2 cells with 0.001, 0.01, 0.1, 1, and 10 µM all-trans-RA. C, untreated; PL, cDNA (CYP26 or $beta$ -actin); M, marker.

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Fig. 8. CYP 26 gene expression in Caco-2 cells measured by RT-PCR. CYP 26, CYP1A1, and $beta$ -actin gene expression was measured under optimal conditions using RT-PCR after treatment of Caco-2 cells with 50 µM $beta$ -naphthoflavone, 10 µM rifampicin, 20 µM all-trans-retinol (in the presence of 6 mM sodium taurocholate), or 10 µM all-trans-RA. C, untreated; NF, $beta$ -naphthoflavone; RIF, rifampicin; ROH, all-trans-retinol; RA, all-trans-RA.

The known inducer of CYP1A1 ( $beta$ -naphthoflavone) failed to induce CYP26 gene expression at all. Furthermore, inducers of CYP3Asuch as rifampicin had no effect on CYP26 gene expression (inCaco-2 cells), indicating the specificity of the induction ofCYP26 by all-trans-RA (Fig. 8). On the other hand, all-trans-RAand all-trans-ROH failed to induce CYP1A1 in Caco-2 cells (Fig.8). CYP1A1 was also induced neither by 9-cis-RA nor by 13-cis-RA(data not shown). Therefore it seems likely that in addition toCYP1A1 and CYP3A, particularly when they are induced by a typicalinducer, CYP26 is the main CYP enzyme responsible for the metabolismof all-trans-RA in Caco-2cells.

	Discussion

Top Abstract Introduction Experimental Procedures Results Discussion References

It is well known that when vitamin A is absorbed in the small intestine, it is converted by ARAT or LRAT into retinyl esters,which are packed in chylomicrons and released into the lymph.We show here for the first time that in the human enterocyte,retinol is oxidized to all-trans-RA and 13-cis-RA. All-trans-RAis further metabolized mainly by CYP26 to more polar metabolitesin Caco-2 cells. It was shown that CYP26 is expressed in humanCaco-2 cells and is inducible by all-trans-RA.

The concentration-dependent formation of the RAR ligands indicates an active saturable enzymatic conversion process in theenterocyte. Enzymes that have been identified in other tissuesthat catalyze the metabolism of retinol to RA were members ofthe family of cytosolic medium-chain ADHs (classes I, II, andIV), aldehyde dehydrogenases (class I), microsomal short-chainADHs (Napoli et al., 1996; Duester, 1996), and CYP1A1 and CYP1A2for the oxidation of retinaldehyde to RA (Tomita et al., 1996).It has also been known that the aldehyde dehydrogen oxidases canconvert retinaldehyde to retinoic acid (Duester, 1996; Napoli,1996). The oxidation of all-trans-retinol to the RAR ligand all-trans-RAby the cytosolic fraction of human small intestinal enterocytesrepresents a new intestinal pathway of vitamin A metabolism. Theinhibition of the formation of RA from dietary ROH by 4-methylpyrazole(an inhibitor of the unspecific ADH) and citral showed that nonspecificADHs as well as aldehyde dehydrogenases may also beinvolved.

The formation of active RAR and RXR ligands in the enterocyte is of particularly interest because retinoic acids (especiallyall-trans-RA) are much more active than retinol. Various studieshave shown that all-trans-RA is essential for proliferation anddifferentiation of epithelial tissues. The human Caco-2 cell linederived from a human colon carcinoma undergoes enterocytic differentiationin culture with morphological (developing microvilli and tightjunctions) and biochemical (increase alkaline phosphatase activity)changes typical for a small intestinal enterocyte (Boulenc etal., 1992; Delie and Rubas, 1997). Caco-2 cells are well establishedin vitro models for the metabolism of CYP1A1 substrates (Boulencet al., 1992) as well as for drug transport (Delie and Rubas,1997). These cells express different CYPs, but only enzymaticcatalytic activities of CYP1A1 and CYP3A have been reported (Boulencet al., 1992; Lampen et al., 1998; Raeissi et al., 1999). Thenuclear retinoid receptors RXR and RAR have been detected in Caco-2cells (McCormack et al., 1996). In Caco-2 cells, RA inhibits growthand stimulates differentiation (McCormack et al., 1996). Incubationof Caco-2 cells with $beta$ -carotene, retinal, or ROH leads to theformation of retinyl esters. The catalytic activities of retinalreductase, ARAT, and LRAT have been detected in microsomal preparationsof Caco-2 cells (Quick and Ong, 1990). Furthermore, it has beenshown that RA induces CRBPII mRNA in Caco-2 cells (Suzuki et al.,1998). Therefore, Caco-2 cells seem to be a valuable model tostudy intestinal metabolism ofretinoids.

In this report we show for the first time that in human intestinal cells (Caco-2), all-trans-RA is formed from dietary vitaminA and further metabolized to the polar metabolites all-trans-4-oxo-RA,all-trans-4-hydroxy-RA, and 13-cis-4-hydroxy-RA. This metabolismis not a simple inactivation because 4-oxo-retinoic acid is believedto be highly active (Pijnappel et al., 1993).

It has long been known that the cytochrome P450 system is active in metabolizing RA. However, a detailed identification ofthe responsible enzymes failed. Our experiments using a specificCYP1A1 inducer ( $beta$ -naphthoflavone) as well as a CYP1A1 inhibitor( $alpha$ -naphthoflavone) suggest an involvement of CYP1A1 in the metabolismof all-trans-RA in Caco-2 cells, provided that CYP1A1 is induced.The incubations with single CYP supersomes showed that CYP3A4,CYP1A1, CYP2C, and CYP2E1 are able to metabolize RA. However,the degree of metabolism was low in comparison with that of specificsubstrates of these cytochromes, suggesting that these cytochromesplay a minor role in intestinal RA metabolism. This interpretationis supported by the observations of Inouye et al. (1999) as wellas by those of Yamazaki and Shimada (1999) who reported a competitiveinhibition of CYP1A1-dependent mono-oxygenase activity by all-trans-RAusing recombinant enzyme systems of rat and human CYP1A1, respectively.These effects seem to be of importance to food toxicological invivo because 2,3,7,8-tetrachlorodibenzo-p-dioxin, a potent CYP1A1inducer, induces increased mobilization of retinoids from hepaticstorage (Brouwer et al., 1989). Furthermore, 2,3,7,8-tetrachlorodibenzo-p-dioxininduces RA metabolism to polar metabolites in liver microsomesof rats (Fiorella et al., 1995). Additionally, aryl hydrocarbonreceptor knockout mice (AHR $-$ / $-$ ) exhibit liver retinoid accumulationand reduced RA metabolism (Andreola et al., 1997). Food contaminantssuch as dioxins and other organohalogen food residues, which arepotent CYP1A1 inducers, may have a significant influence on RAmetabolism and action. On the other hand, all-trans-RA does notinduce CYP1A1 in human Caco-2 cells, although a retinoid-responsiveelement was identified in the promoter region of the human CYP1A1gene (Vecchini et al., 1994). In our study, CYP1A1 was inducedneither by 9-cis-RA nor by all-trans-RA (nor 13-cis-RA), showingthat the CYP1A1 metabolism of RA seems to be a side pathway. Theinduced metabolism of all-trans-RA to all-trans-4-hydroxy-RA afterpretreatment with the CYP3A inducer rifampicin showed that CYP3Ais involved, at least in part, in the metabolism of all-trans-RAin the enterocytes. However, the CYP3A inhibitor ketoconazoleinhibited the metabolism only at high concentrations (>50 µM).

The metabolism of all-trans-RA to polar metabolites was induced by all-trans-RA itself (autoinduction), suggesting that anRA-regulated CYP enzyme is involved. The almost complete inhibitionof the RA metabolism by liarozole and the specific concentration-dependentinduction of CYP26 by retinoids, which seems to correlate withthe concentration-dependent formation of polar metabolites afterincubation of all-trans-RA with Caco-2 cells (Fig. 2B), suggestedthat this could be a main pathway of all-trans-RA. This cytochromeis able to metabolize RA. Both 13-cis- and 9-cis-RA, but not ROH,were found to serve as substrates for CYP26 (Fujii et al., 1997).In adult mice, CYP26 was expressed only in liver (Fujii et al.,1997). When the human cDNA for CYP26 was expressed in COS-1 cells,all-trans-RA was rapidly metabolized to more polar metabolites(all-trans-4-oxo-RA, all-trans-4-hydroxy-RA, and 18-hydroxy-RA).The all-trans-4-oxo-RA and 4-hydroxy-all-trans-RA are also mainmetabolites of intestinal RA metabolism. In the adult human, CYP26is expressed in liver, brain, and placenta (Ray et al., 1997).It was also detected recently in human colon HCT 116 carcinomacells (Sonneveld et al., 1998). We showed that CYP26 is also expressedin human Caco-2 enterocytes and demonstrated its inducibilityby all-trans-RA. Known inducers of other CYPs such as $beta$ -naphthoflavoneand rifampicin did not induce CYP26 gene expression in Caco-2cells at all. Based on the available data, it seems likely thatthe oxidative metabolism of retinoic acid plays an important rolein regulating tissue levels of retinoic acid and that CYP26 mayhave an important role in controlling thismetabolism.

In summary, we report here that the active RAR ligand all-trans-RA is formed in the small intestine via direct oxidation ofvitamin A. In the enterocyte, all-trans-RA is oxidized furtherto polar metabolites mainly through CYP26, which may be an importantregulator of intestinal RA levels. However, CYP1A1 and CYP3A,particularly when induced by $beta$ -naphthoflavone or rifampicin, respectively,seem to participate in part in the metabolism of all-trans-RAin Caco-2cells.

	Acknowledgment

We thank B. Kühlein for technical support of thestudy.

	Footnotes

Accepted for publication July 27, 2000.

Received for publication March 23, 2000.

¹ This work was supported by the European Commission (FAIR CT97-3220).

² Curent address: Boehringer Ingelheim Pharma KG, Biberach,Germany.

Send reprint requests to: Dr. Alfonso Lampen, Zentrumsabteilung für Lebensmitteltoxikologie, Tierärztliche Hochschule Hannover, Bischofsholer Damm 15, D-30173 Hannover, Germany. E-mail: alfonso.lampen{at}tiho-hannover.de

	Abbreviations

LRAT, lecithin-retinol acyl transferase; ARAT, acyl-CoA:retinol-acyltransferase; ADHs, alcohol dehydrogenases; CYP, cytochrome P450; RA, retinoic acid; ROH, retinol; RAR, retinoic acid receptor; RXR, retinoid X receptor; RT-PCR, reverse transcriptase-polymerase chain reaction; nt, nucleotide.

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Metabolism of Vitamin A and Its Active Metabolite All-trans-retinoic Acid in Small Intestinal Enterocytes1

**Metabolism of Vitamin A and Its Active Metabolite All-trans-retinoic Acid in Small Intestinal Enterocytes¹**