©1996 by The American Society for Biochemistry and Molecular Biology, Inc.
In Vitro Metabolism of the Vitamin D Analog, 22-Oxacalcitriol, Using Cultured Osteosarcoma, Hepatoma, and Keratinocyte Cell Lines (*)

(Received for publication, August 25, 1995; and in revised form, January 10, 1996)

Sonoko Masuda (1)(§) Valarie Byford (1) Richard Kremer (2) Hugh L. J. Makin (3) Noboru Kubodera (4) Yasuho Nishii (4) Akira Okazaki (4) Toshio Okano (5) Tadashi Kobayashi (5) Glenville Jones (1)(¶)

From the  (1)Departments of Biochemistry and Medicine, Queen's University, Kingston, Ontario, K7L 3N6 Canada, the (2)Department of Medicine, McGill University, Montreal, H3A 1A1 Quebec, Canada, the (3)Department of Chemical Pathology, The London Hospital Medical College, University of London, London E1 2AD United Kingdom, the (4)Chugai Pharmaceutical Co. Ltd., Tokyo 171, Japan, and the (5)Department of Hygienic Sciences, Kobe Pharmaceutical University, Kobe 658, Japan

ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
FOOTNOTES
REFERENCES

ABSTRACT

Using four cultured cell models representing liver, keratinocyte, and osteoblast, we have demonstrated that the vitamin D analog, 22-oxacalcitriol is degraded into a variety of hydroxylated and side chain truncated metabolites. Four of these metabolic products have been rigorously identified by high pressure liquid chromatography, diode array spectrophotometry, and gas chromatography-mass spectrometry analysis as 24-hydroxylated and 26-hydroxylated derivatives as well as the cleaved molecules, hexanor-1alpha,20-dihydroxyvitamin D(3) and hexanor-20-oxo-1alpha-hydroxyvitamin D(3). Comparison with chemically synthesized standards has revealed the stereochemistry of the biological products. Although differences exist in the amounts of products formed with the different cell types, it is apparent that 22-oxacalcitriol is subject to metabolism by both vitamin D-inducible and noninducible enzymes. Time course studies suggest that the truncated 20-alcohol is derived from a side chain hydroxylated molecule via a hemiacetal intermediate and the 20-oxo derivative is likely formed from the 20-alcohol. Biological activity measurements of the metabolites identified in our studies are consistent with the view that these are catabolites and that the biological activity of 22-oxacalcitriol is due to the parent compound. These results are also consistent with recent findings of others that the biliary excretory form of 22-oxacalcitriol is a glucuronide ester of the truncated 20-alcohol.


INTRODUCTION

It is now firmly established that the hormonal form of vitamin D, 1alpha,25-dihydroxyvitamin D(3) (1alpha, 25-(OH)(2)D(3) or calcitriol) (^1)has potent cell differentiating/anti-proliferative activities in addition to its role in calcium homeostasis(1) . This has led researchers in both universities and the pharmaceutical industry to search for so-called ``noncalcemic'' vitamin D analogs with accentuated differentiating/anti-proliferative properties and reduced ability to cause hypercalcemia(2, 3) . 22-Oxacalcitriol (OCT) (^2)was an early analog developed for this purpose and contains a 22-oxygen atom that replaces the 22-carbon of calcitriol. OCT binds to the chicken vitamin D receptor (VDR) with an approximately 8 times lower affinity than 1alpha,25-(OH)(2)D(3)(4) . However, OCT is 10 times more effective than 1alpha,25-(OH)(2)D(3) in suppressing cell growth and inducing differentiation of the mouse myelocytic leukemic cell, WEHI-3, in vitro(5) . OCT also possesses an enhanced in vivo immunomodulatory potency in mice that is 50 times higher than that of 1alpha,25-(OH)(2)D(3)(6) . In contrast, OCT has reduced calcemic activity in vivo (- that of 1alpha, 25-(OH)(2)D(3)), both in terms of mobilizing calcium from bone and in stimulating intestinal calcium transport in vitamin D-deficient and normal rats(7, 8) . The mechanisms responsible for these differences in biological activity remain unclear, but factors such as cellular uptake and intracellular metabolism could contribute to these differences.

OCT binds poorly to the vitamin D binding protein (DBP) and is transported in the plasma bound by lipoproteins (chylomicrons and low density lipoprotein) in vivo(9) , and this leads to an unusual distribution pattern with a degree of concentration of the vitamin D analog in parathyroid tissue(10) . In contrast, little is known about OCT metabolism except that it appears to be excreted as a glucuronide conjugate in the bile, possibly a derivative of a truncated version of OCT(10) . Furthermore, there have been suggestions that a metabolite with a truncated side chain may be formed in bovine parathyroid cell cultures in vitro(11) , although details of this have yet to be published.

In these studies we set out to provide convincing physicochemical identification for metabolites generated in a variety of cultured cell models, namely the human hepatoma lines HepG2 and Hep3B(12) , the rat osteosarcoma cell line UMR-106(13) , and the human keratinocyte cell lines HPK1A and HPK1A-ras(14, 15) . Because these cell models mimic vitamin D metabolism found in vivo, we expected to observe the same metabolites found and in some cases tentatively identified by others(10, 11) . In addition, our objective was to study the rate of OCT metabolism in various cell lines in order to gauge the involvement of vitamin D-inducible catabolic pathways as compared with more general metabolizing systems. Our results support the concept that OCT is subject to extensive metabolism in a variety of tissues that leads to side chain truncated forms excreted in the bile.


EXPERIMENTAL PROCEDURES

Materials

1alpha,25-(OH)(2)D(3) was a generous gift from Dr. M. Uskokovic of Hoffmann-LaRoche. OCT was synthesized by the method of Murayama et al.(7) . Putative metabolites of OCT, including 22,23, 24,25,26,27-hexanor-1alpha,20-(OH)(2)D(3) and 22,23,24,25,26,27-hexanor-20-oxo-1alpha-hydroxyvitamin D(3) as well as 24- and 26-hydroxylated derivatives, were synthesized as recently described(16) . 25-OH-D(3) and [23,24(n)-^3H]25-OH-D(3) (3.33 TBq/mmol) were obtained from Duphar Co. (Weesp, Holland) and Amersham Corp., respectively. Cell culture media and fine chemicals were purchased from Life Technologies, Inc. Fetal calf serum was from Flow Laboratories (Costa Mesa, CA). Derivatizing agents and solvents were purchased as follows: sodium periodate (BDH Chemicals Ltd, Poole, UK); sodium borodeuteride (Merck, Sharp, & Dohme, Montreal, PQ, Canada); N-trimethylsilylimidazole (Pierce); and HPLC grade organic solvents (Caledon, Georgetown, ON, Canada). All other reagents were analytical reagent grade.

Cell Culture

The cell lines UMR106 and HepG2 were cultured as described previously(12, 13) . Immortalized (HPK1A) and transformed (HPK1A-ras) cell lines were established from normal human keratinocytes by stable transfection with human papilloma virus type 16 followed by transformation with the activated H-ras oncogene, respectively(14, 17) . HPK1A and HPK1A-ras cell lines were cultured as described previously(15) .

Generation of OCT Metabolites

As described previously(15) , 150-mm culture dishes containing monolayers (HPK1A, HPK1A-ras, UMR106, or HepG2) cultured to confluence in the presence of fetal calf serum were washed with phosphate-buffered saline and then incubated in Dulbecco's minimal essential medium containing 1% bovine serum albumin in the presence of 41.8 µg of OCT (10 µM) for 48 h at 37 °C. Except in the time course experiments described below, cells were not treated with 1alpha,25-(OH)(2)D(3) to induce catabolic enzymes. No cell or dead cell controls consisted of 10 ml of medium or microwave-treated cells incubated with OCT under the same conditions for the same length of time. Medium and cells were removed for analysis of OCT metabolites, whereas representative plates of cells were used for determination of cell number using a model ZM automatic cell counter. In the time course study, HPK1A-ras cells were cultured to late log phase in Dulbecco's minimal essential medium containing 10% fetal calf serum and treated with 10 nM 1alpha,25-(OH)(2)D(3) for 16 h in order to maximally induce catabolic enzymes from the beginning. Monolayers were then washed with phosphate-buffered saline containing 2% bovine serum albumin in order to remove residual 1alpha,25-(OH)(2)D(3), and then the medium was changed and the cells were incubated with 41.8 µg of OCT (10 µM) in 10 ml/dish Dulbecco's minimal essential medium containing 1% bovine serum albumin for 0, 1, 3, 6, 12, and 24 h.

Lipid Extraction

Lipid extraction was performed according to the method of Bligh and Dyer (18) as modified by Makin et al.(19) . The organic layer, containing unchanged OCT and lipid-soluble metabolites, was evaporated to dryness, and the residue redissolved in hexane/isopropanol/methanol (HIM), (91:7:2, v/v/v) for straight phase HPLC.

High Performance Liquid Chromatography

Straight phase HPLC was carried out using a model 590 pump, a U6K manual injector, and a model 990 photodiode array detector (all from Waters Associates, Milford, MA). This scanning spectrophotometer was used during metabolite purification to identify peaks possessing UV characteristics of the vitamin D cis-triene system (UV(max) = 265 nm, UV(min) = 228 nm, UV = 1.75). Separations were achieved using Zorbax SIL (6.2 times 80 mm) or Zorbax CN (4.6 times 250 mm) columns (Dupont NEN). Mobile phases used for OCT metabolites included mixtures of HIM ranging from 91:7:2 to 94:5:1. Concentrations of stock solutions of OCT and its metabolites were assessed spectrophotometrically using a molar extinction coefficient, = 18,300.

Purification of Metabolites

The lipid residue from the extraction of three 150-mm culture dishes containing HPK1A-ras (or HPK1A) cells was redissolved in 1.2 ml of HIM 91:7:2. Initial chromatography was performed on Zorbax SIL using HIM 91:7:2 at flow rate 1.0 ml/min. Six 200-µl aliquots of the extract were chromatographed, and peaks possessing the characteristic chromophore of vitamin D were collected and pooled. These fractions were subjected to further chromatography on Zorbax CN and Zorbax SIL. At this point, metabolites were pure enough for chemical derivatization and/or mass spectrometry.

Derivatization Reactions

Periodate oxidation and borohydride reduction of metabolites of OCT were carried out according to published methods(13, 20) .

Gas Chromatography-Mass Spectrometry

Purified metabolites were derivatized to pertrimethylsilyl ethers and then analyzed by GC-MS as described previously(20) . Injection of metabolites of OCT into the high temperature injection zone of the GC causes B ring closure producing pyro- and isopyroisomers. Mass spectra were obtained only from the pyroisomer, and, for simplicity, in discussion of fragmentation and in figures illustrating spectra obtained, the uncyclized metabolite structure is used rather than that of the correct pyroisomer. Mass spectra were obtained by averaging each peak and subtracting the background.

Biological Properties of OCT and Its Metabolites

VDR Binding Assay

The binding affinities of OCT and its metabolites for the calf thymus vitamin D receptor were tested using a 1alpha,25-(OH)(2)D(3) assay kit purchased from INCSTAR (Stillwater, MN). Calf thymus VDR was incubated at 20 °C for 1 h with various concentrations of 1alpha,25-(OH)(2)D(3) (1.25-80 pg/tube), OCT (1.25-80 pg/tube), or its metabolites (2.5 pg/tube to 205 ng/tube). After the incubation period, 15,000 dpm of [^3H]1alpha,25-(OH)(2)D(3) was added and incubated for 1 h at 20 °C. Bound and free forms of [^3H]1alpha,25-(OH)(2)D(3) were separated by addition of a dextran/charcoal suspension and centrifugation. Radioactivity was measured with an Aloka LSC-90.

DBP Binding Assay

The binding affinities of OCT and its metabolites for the DBP were tested using plasma from a vitamin D-deficient rat. The displacement of [^3H]25-OH-D(3) from 1:70,000 diluted vitamin D-deficient rat plasma in 3.5 mM barbiturate buffer (pH 8.6) containing 0.13 M NaCl and 0.1% ovalbumin was measured following the addition of 25-OH-D(3) (12.5 pg/tube -3.2 ng/tube), 1alpha,25-(OH)(2)D(3) (1.6-820 ng/tube), or OCT or its metabolites (51 ng/tube to 52.4 µg/tube) as described previously(21) . After incubation for 1 h at 4 °C, bound and free forms of [^3H]25-OH-D(3) were separated by the addition of a dextran/charcoal suspension and centrifugation. The supernatants containing bound [^3H]25-OH-D(3) were transferred into scintillation vials, and radioactivity was measured in a scintillation counter.

Assessment of Cell Growth of HL-60(22

Human promyelocytic leukemic cells (HL-60 cells) were kindly provided by Dr. M. Inaba (Osaka City University, Medical School). Cells were cultured at 37 °C in RPMI 1640 medium (Nissui Pharmaceutical, Japan) supplemented with 10% heat-inactivated fetal calf serum and 60 µg/ml of kanamycin in a humidified atmosphere of 5% CO(2) in air. Under these conditions the doubling time of HL-60 cells was 24 h. Vitamin D treatment involved seeding HL-60 cells at 1 times 10^5 cells/ml in growth medium and culturing for 72 h in the presence of from 10M to 10M of 1alpha,25-(OH)(2)D(3), OCT, or its metabolites, each dissolved in ethanol. Control cultures were treated with ethanol vehicle at 0.1% (v/v). After the incubation period, cells were harvested, and the cell number was determined using a hemocytometer. Cell viability was determined by trypan blue exclusion. The number of cells counted from triplicate experiments was expressed as a percentage of the control. The results are expressed as the mean of triplicate counts ± standard error.


RESULTS

Metabolism of OCT in the Human Keratinocyte Cell Line, HPK1A-ras

In an attempt to establish the full extent of metabolism of OCT, we began our studies by incubating this analog with the cell line HPK1A-ras, previously shown to have very high catabolic activity toward 1alpha,25-(OH)(2)D(3)(15) . When we incubated 10 µM OCT for 48 h, we obtained extensive metabolism such that on HPLC seven metabolite peaks possessing the vitamin D chromophore were discernible. These are labeled peaks 1-7 in Fig. 1, where peak 3 is the substrate, OCT, and the rest are metabolic products. Little substrate was left at the end of the 48-h period, whereas no metabolites were formed in no cell or dead cell (microwave-treated) control plates incubated with OCT (Fig. 1A). All peaks 1-7 were purified by extensive rechromatography on Zorbax-CN and then again on Zorbax-SIL in order to identify them by GC-MS and chemical derivatization. In the case of peak 2, we made a sodium borodeuteride reduction product and an oxime as well as the pertrimethylsilylated derivative. In the case of peaks 4, 6, and 7, they were subjected to GC-MS as the pertrimethylsilylated derivatives or, in the case of peaks 6 and 7, as their n-butyl boronate ester/pertrimethylsilylated derivatives.


Figure 1: HPLC of extract of HPK1A-ras cells incubated with 10 µM OCT for 48 h. Peaks showing the vitamin D chromophore are numbered 1-7. A shows the no cell control experiment. B shows the extract from HPK1A-ras cells. the HPLC conditions were Zorbax-SIL (3 µ; 6.2 times 80 mm); HIM 91:7:2, 1.0 ml/min.



Identification of the Major Metabolites of OCT

We have summarized in Table 1and detailed below the evidence that was obtained for the successful identification of the major metabolites. Peak 3 was identified as unchanged substrate. We obtained limited information regarding peaks 1 and 5, and these metabolites remain unidentified at this time.



Peak 2 (22,23,24,25,26,27-Hexanor-20-oxo-1alpha-hydroxy vitamin D(3)

This peak ran at 10.72 min, slightly ahead of the substrate OCT (RT = 11.41 min) on Zorbax-SIL chromatography. Peak 2 was significantly retarded relative to OCT on Zorbax-CN chromatography (see Table 1), suggesting the presence of a C=O group in the molecule. The pertrimethylsilylated derivative of peak 2 showed a molecular ion at m/z 474 on GC-MS (Fig. 2A), suggesting truncation of the side chain between the 22-oxa-group and the C-23 and retention of the 22-oxa group as a 20-ketone functionality with the subsequent addition of only two TMS groups. The remainder of the mass spectrum with major ions at m/z 384(474 - 90), 343 (loss of a fragment containing carbons C-2,3,4), 294(474 - 90 - 90), and 217 (loss of a fragment containing carbons C-1,2,3) was consistent with this interpretation.


Figure 2: A, mass spectrum of pertrimethylsilylated peak 2. B, mass spectrum of pertrimethylsilylated oxime derivative of peak 2.



Treatment of peak 2 with sodium borodeuteride gave two product peaks, one of which co-migrated with peak 4 (peak 2 (untreated) = 10.77 min; peak 2 treated with NaBD(4) product 1 = 12.88 min and product 2 = 14.94 min; peak 4 (untreated) = 14.91 min using Zorbax-SIL, HIM, 91:7:2 1 ml/min). When the NaBD(4) reduction product of peak 2 was further derivatized with N-trimethylsilylimidazole, the pertrimethylsilylated product gave a molecular ion of m/z 549 (Fig. 3B) corresponding to the addition of one deuterium atom to the original molecule and fragments at m/z 459(549 - 90), 418 (549 - 131 due to loss of a fragment containing carbons C-2,3,4), 369(549 - 90 - 90), and a base fragment of m/z 118 corresponding to cleavage of the C-17-C-20 bond. This spectrum is very similar to that of peak 4 and is consistent with the reduction of the 20-ketone to a mixture of monodeuterated 20-alcohols.


Figure 3: A, mass spectrum of pertrimethylsilylated peak 4. B, mass spectrum of pertrimethylsilylated derivative of the sodium borodeuteride reduction product of peak 2.



Final proof of the identity of peak 2 as the 20-ketone came from formation of an oxime derivative. When the oxime was further derivatized with N-trimethylsilylimidazole, it gave a pertrimethylsilylated derivative with a molecular ion of m/z 503 (Fig. 2B). Major fragment at 413 (M-90), 382 (M-OCH(3)-90), 370 (M-131 due to loss of a fragment containing carbons C-2,3,4), and 292 (M-OCH(3)-90-90) are all consistent with a 20-oxime derivative. We conclude from HPLC, GC-MS, borohydride reduction, and oxime formation that peak 2 is the truncated 20-ketone.

Peak 4 (22,23,24,25,26,27-Hexanor-1alpha,20-dihydroxyvitamin D(3))

Peak 4 was more strongly retained than OCT at 14.91 min on Zorbax-SIL chromatography. Peak 4 co-migrated with synthetic hexanor-1alpha,20S-dihydroxyvitamin D(3) on both Zorbax-SIL and Zorbax-CN. GC-MS of the pertrimethylsilylated derivative of peak 4 gave the mass spectrum shown in Fig. 3A and can be seen to be homologous to the monodeuterated peak 2 (Fig. 3B). Pertrimethylsilylated peak 4 possessed a molecular ion of m/z 548 corresponding to a C sterol with three TMSOH groups. The fragmentation pattern shows the expected features with m/z 458 (M - 90), 368 (M - 90 - 90), and 417 (M - 131 due to loss of a fragment containing carbons C-2,3,4), but in addition, a fragment at m/z 117 corresponding a C(2) fragment from C-20 and C-21 bearing a TMS group. We conclude peak 4 is the truncated 20-alcohol derivative of OCT.

Peak 6 (24-Hydroxy-OCT)

This peak was the major product of all the cell types tested, and because all are known to be rich sources of 24-hydroxylase activity, it seemed logical that peak 6 would prove to be the 24-hydroxy derivative of OCT. A moderately polar peak on Zorbax-SIL, this peak was sensitive to sodium metaperiodate treatment, suggesting the presence of vicinal hydroxyl functions at C-24 and C-25. On GC-MS (Fig. 4A) the pertrimethylsilylated derivative of peak 6 possessed a molecular ion of m/z 722 with major fragments at 632 (M - 90) and 542 (M - 90 - 90) as well as m/z 591 (M - 131 due to loss of a fragment containing carbons C-2,3,4) and m/z 459, 369, and 279 found in the original substrate, suggesting no alteration of the ring structure. The base peak at m/z 131 is indicative of retention of the C-25 hydroxyl function intact.


Figure 4: A, mass spectrum of pertrimethylsilylated peak 6. B, mass spectrum of pertrimethylsilylated derivative of the n-butyl boronate ester of peak 6.



The n-butylboronate derivative of peak 6 was formed, again suggesting vicinal hydroxyls at C-24 and C-25. The pertrimethylsilylated n-butyl boronate of peak 6 gave the mass spectrum (Fig. 4B) with the predicted molecular ion of m/z 644 and a fragmentation pattern particularly m/z = 169 due to cleavage of the oxygen O-22-C-23 bond consistent with a 24-hydroxylated precursor. Finally, peak 6 was shown to co-chromatograph with chemically synthesized 24R-OH-OCT on HPLC. We conclude on the basis of extensive evidence that peak 6 is 24R-hydroxy-OCT.

Peak 7 ((25R)-26-Hydroxy-OCT)

This peak was the most polar metabolite obtained with a retention time of 23.99 min on Zorbax-SIL and 16.73 min on Zorbax-CN (Table 1). Like peak 6, it proved to be sensitive to sodium metaperiodate, giving a product with a much reduced retention time (12.13 min versus OCT = 11.35 min). On GC-MS, the pertrimethylsilylated derivative of peak 7 gave a molecular ion of m/z 722, suggesting a monohydroxylated derivative of OCT. The mass spectrum (Fig. 5A) featured many of the same ions found in the spectrum of peak 6 except that there was a large fragment at m/z 103 (corresponding to loss of CH(2)OTMS) instead of m/z 131 found in the case of 24-hydroxy-OCT. This fragment is indicative of a CH(2)OTMS presumably vicinal to the existing C-25 hydroxy group at C-26 (C-27).


Figure 5: A, mass spectrum of pertrimethylsilylated peak 7. B, mass spectrum of pertrimethylsilylated derivative of the n-butyl boronate ester of peak 7. C, mass spectrum of pertrimethylsilylated derivative of the sodium periodate cleavage product of peak 7.



On GC-MS, the periodate cleavage product of peak 7 gave no discernible molecular ion, but the fragmentation pattern featured large fragments at m/z 456 (M - 90) and 366 (M - 90 - 90) and m/z 415 (M - 131 due to loss of a fragment containing carbons C-2,3,4), data consistent with the molecular ion being extrapolated to be m/z 546 (Fig. 5C). This is consistent with a molecule truncated between C-25 and C-26 (C-27) and containing a C-25 ketone. Further confirmation of the peak 7 being a molecule with vicinal hydroxyls came from formation of an n-butylboronate derivative. As with peak 6 the pertrimethylsilylated version of this was subjected to GC-MS and gave a molecular ion of m/z 644 (Fig. 5B). In addition to the distinctive fragment at m/z 169 found with the n-butylboronate, pertrimethylsilylated derivative of 24-hydroxy-OCT, we observed a distinctive fragment at m/z 141 due to cleavage of the C-24-C-25 bond and loss of a fragment containing the C-25, C-26, and C-27 butylboronate ester group. Finally, peak 7 was shown to co-chromatograph with chemically synthesized (25R)-26-OH-OCT on HPLC. We conclude from these data that peak 7 must be (25R)-26-hydroxy-OCT.

Comparison of Biological Products to Chemically Synthesized Standard Compounds

As a result of preliminary in vitro studies, both possible epimers of each biologically generated metabolite were synthesized chemically. Table 2shows the results of HPLC co-migration studies of biological and chemically synthesized metabolites. In each case the epimeric mixture could be resolved on HPLC, and the biological product was found to be exclusively one epimer (that is peak 4 = 20S-epimer of the hexanor-1alpha,20-(OH)(2)D(3), peak 6 = 24R-hydroxy OCT, and peak 7 = 25R-form of 26-hydroxy OCT). All chemically synthesized standard compounds were subjected to GC-MS for comparison to previously obtained mass spectra of biological products. Mass spectra (data not shown) were found to be virtually identical to those shown in Fig. 2Fig. 3Fig. 4Fig. 5and therefore corroborate the identifications provided.



Time Course of OCT Metabolism in HPK1A-ras Cells

Evidence from the time course suggests that at early time points the hexanor-1,20-(OH)(2)D(3) is present when there is no detectable hexanor-20-oxo-1alpha-OH-D(3) (Fig. 6). All other metabolites accumulate at early time points, and their concentration plateaus or even decreases by the end of the incubation period (24 h).


Figure 6: Time course of OCT metabolism in HPK1A-ras cells.



Studies of the Metabolism of OCT in the HPK1A Keratinocyte, the Rat Osteosarcoma, UMR-106, and the Human Hepatoma, HepG2

In these studies we examined the metabolism of OCT using established cell lines involved in both the activation and catabolism of vitamin D. With such cell lines it was found that OCT was metabolized to a smaller number of products, which comigrated with peaks 4, 6, and 7 obtained using HPK1A-ras (Fig. 7). Metabolites were subjected to the same rigorous identification used for those from HPK1A-ras.


Figure 7: HPLC of extract of other cell lines incubated with 10 µM OCT for 48 h. A, HPK1A cells. B, UMR-106 cells. The HPLC conditions are as described in the Fig. 1legend.



When we compared metabolism of OCT at the same time, under the same experimental conditions (Fig. 8), we confirmed that OCT had virtually disappeared at the end of the 48-h period in HPK1A-ras cells, whereas considerable amounts remained in plates containing UMR-106 and HPK1A cells. The major metabolite found in cell cultures of UMR-106 and HPK1A was the 24-hydroxy-OCT (peak 6), whereas the truncated metabolites, peaks 4 and 2, appeared to be more important as the degree of metabolism increased (e.g. in HPK1A-ras). These data are consistent with the scheme shown in Fig. 9with monohydroxylated versions of OCT acting as intermediates to the truncated metabolites, peaks 4 and 2.


Figure 8: Amounts of metabolites formed from OCT in various cultured cell lines. The results are expressed as the total amount of product formed (and thus isolated) in µg/48 h. The amount of OCT remaining in the cultures was 1.4 µg for HPK1A-ras, 26 µg for HPK1A, and 28.5 µg for UMR106 and was not determined for Hep G2.




Figure 9: Proposed pathway of OCT metabolism in cultured vitamin D target cells in vitro.



Biological Activities of OCT and Its Metabolites

The VDR binding affinities of the 26-hydroxy-OCT isomers (ED141 and ED142) or side chain truncated metabolites of OCT (ED26, ED190, and ED67) were much reduced compared with the parent molecule, OCT, which showed approximately the same binding affinity for the mammalian VDR as 1alpha,25-(OH)(2)D(3) (Fig. 10A). This was especially true of the side chain truncated metabolites of OCT, which showed a binding affinity 2-3 orders of magnitude lower than 1alpha,25-(OH)(2)D(3). On the other hand, 24R-hydroxy-OCT (ED106) or 24-oxo-OCT (ED174) retained much of the VDR-binding affinity of OCT with values only - that of OCT, respectively.


Figure 10: Biological activity of the metabolites of OCT (relative to 1alpha, 25-(OH)(2)D(3)). A, VDR binding. B, DBP binding. C, inhibition of HL-60 cell growth. For clarity, only the chemically synthesized epimer corresponding to the biologically generated metabolite is illustrated. The biological activity of the other epimer was determined, and the data are depicted numerically in Fig. 11. circle, 1alpha,25-(OH)(2)D(3); bullet, OCT; up triangle, 24R-OH-OCT; box, (25R)-26-OH-OCT; , hexanor-20-oxo-1alpha-OH-D(3); down triangle, hexanor-1alpha,20S-(OH)(2)D(3).




Figure 11: Structures and biological activity data for chemically synthesized metabolites of OCT. The data are summarized for both stereochemical versions of each metabolite.



The measurements of the DBP-binding affinity (Fig. 10B) confirmed earlier observations (4, 9) that OCT showed a value 2 orders of magnitude lower than 1alpha,25-(OH)(2)D(3) and 4 orders of magnitude lower than 25-OH-D(3) (data not shown). No metabolite of OCT possessed a higher affinity for DBP than OCT.

In the growth response study (Fig. 10C), 1alpha,25-(OH)(2)D(3) suppressed cell growth of HL-60 in a dose-dependent manner when used at a concentration between 1 times 10M and 1 times 10M. Significant inhibition of growth could be seen at a steroid concentration as low as 10M 1alpha,25-(OH)(2)D(3) where the growth was decreased to <40% of control. The suppression of cell growth provided by OCT was virtually identical, whereas the suppressions caused by the hexanor-20-oxo-compound (ED26) or the hexanor-20S-hydroxy- compound (ED67) were greater than 2 orders of magnitude less effective than 1alpha,25-(OH)(2)D(3). Other metabolites such as 24R-hydroxy-OCT (ED106) or (25R)-26-hydroxy-OCT (ED141) showed slightly inferior growth-inhibiting activity to OCT, with potencies between and that of 1alpha,25-(OH)(2)D(3). The results of the biological activity studies for all chemically synthesized epimers, including biologically generated products of OCT, are summarized in Fig. 11.


DISCUSSION

We have described here the extensive metabolism of the vitamin D analog, 22-oxacalcitriol in a variety of cultured cell lines, including one hepatoma cell line and three vitamin D-target cell lines previously shown to catabolize 1alpha,25-(OH)(2)D(3). Our study is the first to rigorously identify any of the metabolic products of OCT formed in vitro, and this was made possible by the generation of microgram quantities of these metabolites. The novel metabolites identified include two truncated versions of the OCT molecule lacking carbons 23-27 and containing a 20-oxo or 20-hydroxyl group. The 20-hydroxy compound has been reported before in vitro, but identification was based solely upon comigration with a chemically synthesized standard on HPLC(11) . Here we were able to augment the preliminary identification afforded by HPLC co-chromatography with GC-MS analysis and later comparison with chemically synthesized standards. Furthermore, our work is also consistent with the preliminary finding of a glucuronide conjugate of the 20-hydroxy compound in rat bile following OCT administration(10) . The 24R-OH-OCT and 26-OH-OCT in the 25R-form identified here are novel, and their stereochemistry is also established.

The finding of both intact and truncated versions of OCT in cell extracts evokes the obvious question of how is OCT cleaved? Our venture into the metabolic fate of an oxygen containing molecule was not without precedent. In a previous study, we examined the metabolic fate of 24-oxa-1alpha-OH-D(3) in the same hepatoma cell line HepG2 (23) . In that case, we also found cleaved molecules, although the ultimate products were 23-substituted and lacked the carbon atoms C-25, C-26, and C-27 of the starting material. Thus, in the cases of both 22-oxacalcitriol and 24-oxa-1alpha-hydroxyvitamin D(3), the molecule is cleaved just distal to the oxygen atom. In the case of 24-oxa-1alpha-OH-D(3), we hypothesized that the enzymatic hydroxylation of a carbon vicinal to the oxygen atom would give rise to an unstable hemiacetal linkage that would undergo spontaneous breakdown to the C-23 substituted products(23) . If we extrapolate from this result to the case of OCT we would predict that C-23 hydroxylation would have to occur in order to generate an unstable hemiacetal and truncated products retaining the 22-oxa group. The metabolites that were observed, namely 24-OH-OCT and 26-OH-OCT, would appear to be either precursors to this 23-hydroxylated intermediate or are by-products of the metabolic machinery. It is interesting to note that a 24-hydroxylated version of 1alpha,25-(OH)(2)D(3) precedes a 23-hydroxylated metabolite in the catabolic sequence for the natural hormone during its conversion to calcitroic acid observed in a variety of target cell systems(19, 24) . Alternatively, others have identified 26-hydroxylated derivatives of 25-OH-D(3)(25) and 1alpha,25-(OH)(2)D(3)(26) and a 26-hydroxylated metabolite is observed as an intermediate during formation of the 26,23-lactone, but this is postulated to occur after and not prior to 23-hydroxylation(27) . It remains to be proven if either 24-OH-OCT or 26-OH-OCT is a precursor to the 20-hydroxy and 20-oxo derivatives also found here.

Only in the case of the keratinocyte cell lines (HPK1A-ras and HPK1A) did we find appreciable quantities of the 20-oxo-truncated derivative of OCT. It is possible that the pattern of OCT metabolism that we observed, including the formation of the 20-oxo derivative, resulted from the induction of the catabolic enzymes caused by the high substrate concentrations that we employed. Interestingly, we observed the same pattern of metabolites including the 20-hydroxy and 20-oxo-truncated derivatives when [2beta-^3H]OCT (12 Ci/mmol) was incubated at low nanomolar concentrations with HPK1A-ras cells (data not shown). The formation of the 20-oxo derivative could also be due to the different redox state of these cells compared with the other cell lines used. On the other hand, this may provide evidence of the role of one compound as an intermediate in the formation of the other (see Fig. 9). The time course study carried out suggests that the 20-hydroxy compound predates the 20-oxo derivative and thus may be converted to the latter in this culture system.

The biological activities of the metabolites identified here (where possible together with their epimeric forms; see Fig. 11) provides evidence that the in vivo properties of OCT can probably be ascribed to the parent compound and not to its principal products. In all cases, metabolites of OCT were inferior to OCT (and 1alpha,25-(OH)(2)D(3)) in all parameters measured (i.e. VDR binding, DBP binding, and growth suppression of HL-60). This was particularly marked for the 20-oxo and 20-hydroxy derivatives where truncation of the side chain of OCT lowered biological activity by more than 2 orders of magnitude. A rough correlation between the strength of calf thymus VDR binding and the ability of the vitamin D analog to inhibit growth of HL-60 cells was still discernible. As with other 22-oxa analogs studied in this field (e.g. 28), the calcium-transporting activity of the metabolites reported here remains unknown.

In the work described here, we observed OCT metabolism in both vitamin D target cells, namely, bone and keratinocyte, as well as a tissue involved in the activation of vitamin D, namely liver. It has been previously shown that like 1alpha,25-(OH)(2)D(3) metabolism(19) , OCT metabolism is vitamin D-inducible in cultured bovine parathyroid cells (11) and normal human peripheral monocytes (29) . The result that hepatoma cells are also able to form truncated OCT metabolites is interesting given that liver cells are thought to be devoid of the vitamin D receptor and the vitamin D-inducible catabolic enzymes (e.g. cytochrome P-450 CYP24)(30, 31) . However, small modifications of the vitamin D side chain have been shown to result in much more rapid hepatic metabolism and indeed 24-hydroxylation and 24-oxidation of certain analogs (e.g. calcipotriol)(32, 12, 15) . Thus, it is possible that in addition to being susceptible to attack by vitamin D-inducible enzymes in classical vitamin D target cells, OCT is also attacked by more general enzymes in the liver leading to cleavage of the side chain by similar or slightly different mechanisms. It is clear from the studies presented here that OCT is more efficiently degraded by vitamin D-target cells than by hepatoma cells, and this may be important to the in vivo distribution and biological activity of the drug (33) as well as to the endogenous ligand(34) .

Lastly, our finding of truncated versions of OCT would seem to open the door to study the origin of the conjugates found in bile in vivo following OCT administration to rats(10) . The free 20-oxo or 20-hydroxy compounds identified here would likely be transported to the liver prior to conjugation to glucuronic acid in the hepatocyte, but this remains to be proven.


FOOTNOTES

*
This work was partially supported by grants from the Medical Research Council of Canada (to G. J.). The costs of publication of this article were defrayed in part by the payment of page charges. This article must therefore by hereby marked ``advertisement'' in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.

§
Recipient of a John Alexander Stewart Fellowship, Department of Medicine, Queen's University.

To whom all correspondence should be addressed. Fax: 613-545-2987.

(^1)
D(2) and D(3) indicate vitamins D(2) and D(3), respectively, and OH and (OH)(2) indicate hydroxy and dihydroxy, respectively. Therefore, for example, 1alpha,25-(OH)(2)D(3) represents 1alpha,25-dihydroxyvitamin D(3).

(^2)
The abbreviations used are: OCT, 22-oxacalcitriol; DBP, vitamin D binding protein (Gc-globulin); HIM, hexane/isopropanol/methanol; VDR, vitamin D receptor; HPLC, high pressure liquid chromatography; GC-MS, gas chromatography-mass spectrometry; TMS, trimethylsilyl.


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