Abstract
In experiments with expressed human UDP-glucuronosyltransferase 1A4 (UGT1A4), the antipsychotic clozapine proved to be conjugated to two different glucuronides, one of which was identified as the quaternary ammonium glucuronide derivatized at theN-methylpiperazine group; this compound had previously been isolated from patient urine. An additional glucuronide produced in larger quantity was assumed to be conjugated at the secondary nitrogen of the central ring to form 5-N-glucuronide, but this was not proven. The analogous olanzapine 10-N-glucuronide was found to make a major contribution to urinary metabolites in human volunteers. In the present investigation, tertiary 5-N-glucuronides were isolated from incubations of clozapine and desmethylclozapine with human liver microsomes fortified with UDP-glucuronic acid, and their structures were confirmed by mass and 1H NMR spectrometry. The same conjugates could also be purified from patient urine. Their approximate quantities in urine from four patients ranged between 0.1 and 0.5% of the dose, as did those of the quaternary ammonium glucuronide of clozapine. Analogous to olanzapine 10-N-glucuronide, the tertiary clozapine 5-N-glucuronide was resistant toward enzymatic hydrolysis but was labile under acidic conditions.
The atypical antipsychotic clozapine is known to undergo a large number of biotransformation reactions in humans. Most of these are oxidative and comprise N-demethylation,N-oxidation (Gauch and Michaelis, 1971), aromatic hydroxylation, and exchange of aromatically bound chlorine against hydroxy or methylthio groups (Stock et al., 1977; Dain et al., 1997;Schaber et al., 2001). In addition, analyses of patient urine and experiments in vitro have revealed the possibility of direct conjugation of clozapine at nitrogen atoms. Luo et al. (1994) succeeded in isolating from patient urine clozapineN+ -glucuronide, the quaternary ammonium glucuronide resulting from conjugation at theN-methylpiperazine group. Its mass spectrum was identical with that of a synthetic reference compound. The same glucuronide was the minor product when clozapine was incubated with expressed human UGT1A4 in the presence of UDP-glucuronic acid (Green and Tephly, 1996). For the major conjugate, structural proof was not possible, but glucuronic acid attachment at the secondary nitrogen (N-5) of the central ring was suggested because an analogous conjugate was not formed from loxapine in which the secondary nitrogen is lacking. The assumption became more probable when the biotransformation of olanzapine, an atypical antipsychotic closely related to clozapine, was investigated in human volunteers (Kassahun et al., 1997). In urine and feces, a tertiary N-glucuronide, 10-N-glucuronide, was found to be a major metabolite, whereas a quaternary ammonium glucuronide represented a smaller fraction of the dose. The authors reported that the quaternary, but not the tertiary N-glucuronide, could be hydrolyzed enzymatically, whereas the latter was acid-labile.
The present experiments were performed to answer the question whether glucuronidation at the secondary nitrogen atom plays a part in the metabolic fate of clozapine in vivo. For this purpose, unambiguous identification of the tertiary 5-N-glucuronides of clozapine and desmethylclozapine was achieved by their isolation from incubates with human liver microsomes and patient urine and measurement of their mass and NMR spectra. A procedure was developed for the quantitation of the tertiary and quaternary N-glucuronides in patient urine, and the susceptibility of clozapine 5-N-glucuronide toward enzymatic and acid hydrolysis was investigated.
Experimental Procedures
Substances.
Clozapine and N-desmethylclozapine were kindly provided by Novartis (Basel, Switzerland). The disodium salt of UDP-glucuronic acid and β-glucuronidase from E. coli K 12 were purchased from Roche Diagnostics (Mannheim, Germany), β-glucuronidase from Helix pomatia was obtained from Sigma (Deisenhofen, Germany). Clozapine N+ -glucuronide was prepared by a modification (Schaber et al., 2001) of the procedure ofLuo et al. (1992).
Preparation of N-Glucuronides by Microsomal Incubation.
Human liver microsomes prepared by conventional methodology (Breyer-Pfaff and Nill, 1995) were incubated for 1 h at 37°C at 1 mg/ml with (final concentrations) 25 mM saccharose, 50 mM Tris-HCl, pH 8.0, 10 mM MgCl2, 2 mM UDP-glucuronic acid, and 0.5 mM clozapine or desmethylclozapine in a total volume of 3 ml. After cooling, protein was precipitated with 0.3 ml of 150 mM barium hydroxide, followed by 0.3 ml of 150 mM zinc sulfate. From the supernatant, unreacted drug was largely removed by extraction with 1 and 2 ml of tert-butylmethylether in the case of clozapine and by three extractions with 3 ml in the case of desmethylclozapine. Following extraction with 1 ml of hexane, the aqueous solution was passed through a cartridge with 100 mg of C18-silica gel (Bond Elut; Analytichem International, Harbor City, CA). After washing with 1.5 ml of water, adsorbed compounds were eluted with 1.5 ml of methanol and 1.5 ml of methanol/25% ammonia (9:1, v/v). The combined organic phases were evaporated, and the residue was subjected to thin layer chromatography in 1-butanol/acetone/25% ammonia/water (2.5:2.5:1:0.5, v/v) on sheets precoated with silica gel with a fluorescent indicator (Alugram Sil G/UV254; Macherey-Nagel, Düren, Germany). When clozapine had been incubated, a weak UV-absorbing band was present atRF 0.3 (identical with theRF of clozapineN+ -glucuronide) and a stronger band atRF 0.52 assumed to contain the tertiaryN-glucuronide. In extracts from incubations of desmethylclozapine, the substrate was present atRF 0.77, and an additional band probably containing N-glucuronide was present atRF 0.46. The glucuronide bands were removed and extracted three times with 2 ml of methanol. The extract residues were homogeneous in HPLC1; for NMR and mass spectrometry, the extracts were dissolved in water, adsorbed on C18-silica gel cartridges, eluted with methanol, and evaporated.
For an estimate of the quantity formed, the UV spectrum of an aliquot of the purified compound was measured in methanol and compared with that of clozapine at a defined concentration. The quantities per milliliter of incubate were about 20 nmol of clozapine 5-N-glucuronide, 5 nmol of clozapineN+ -glucuronide, and 5 nmol of desmethylclozapine 5-N-glucuronide.
Isolation of Tertiary N-Glucuronides from Urine.
Urine was obtained from a male patient of 31 years who received 400 mg/day clozapine as a monotherapy and had serum concentrations of 331 ng/ml clozapine and 283 ng/ml desmethylclozapine. Of the 24 h-sample of 3050 ml, an aliquot of 500 ml was applied to a C18-silica gel column (150 × 10 mm; Polygosil 40 to 63 μm; Macherey-Nagel) pretreated with methanol/25% ammonia (9:1) and water. The column was washed with 75 ml of water and 25 ml of 1% ammonia; adsorbed substances were eluted with 75 ml of methanol and 25 ml of methanol/25% ammonia (95:5). The eluate was evaporated under reduced pressure, dissolved in 10 ml of water, and after adjusting pH to 9 to 10 with ammonia, extracted three times with 10 ml of tert-butylmethylether and once with hexane for removal of unpolar compounds. The aqueous phase was again applied to C18-silica gel (5 ml), followed by washing with water and elution with methanol (8 ml), methanol/25% ammonia (9:1, 4 ml), and methanol (4 ml). The eluate was evaporated, and the residue dissolved in 1.5 ml of methanol. Fractions of 0.3 ml were separated by thin layer chromatography on 20- × 20-cm silica gel sheets in 1-butanol/acetone/25% ammonia/water (5:5:1.5:0.5, v/v). The bands corresponding to clozapine 5-N-glucuronide (RF 0.31) and desmethylclozapine 5-N-glucuronide (RF 0.22) from microsomal incubations were removed and extracted three times with 2 ml of methanol. On rechromatography in ethanol/water/triethylamine (9:0.6:0.4, v/v), clozapine 5-N-glucuronide was found atRF 0.64 and its demethylated analog atRF 0.39. Further purification was achieved in 1-butanol/acetone/ammonia/water (5:5:2:1, v/v) withRF values of 0.53 and 0.39, respectively. Finally, semipreparative HPLC in system 1 served to purify about 400 μg of clozapine 5-N-glucuronide in three fractions and about 70 μg of the desmethyl analog in one fraction. The eluates were alkalinized with ammonia and evaporated under reduced pressure. The twoN-glucuronides then were homogeneous (except for admixtures of the aglycones) and identical in HPLC with reference compounds produced by microsomes. Before structural elucidation, they were purified by adsorption to C18-silica gel and elution with methanol, as described above. In the final step of preparation and during the storage of solutions in methanol or water at 4°C, slow decomposition took place such that an admixture of unconjugated drugs of 5 to 15% could not be avoided.
Measurement of N-Glucuronides in Urine.
Three additional patients receiving clozapine monotherapy for at least 4 weeks collected urine. In two cases, 24 h-sampling was not possible, but the time of urine collection was noted. Aliquots of 10 ml were adjusted to pH 6.5 to 7 by ammonia, centrifuged, and extracted on Bond Elut cartridges containing 100 mg of C18-silica gel. After washing with 1.5 ml of water, elution was carried out with 1.5 ml of methanol. The eluate was evaporated at 35°C, and unpolar compounds were removed by distribution between 0.2 ml of 100 mM Tris-HCl buffer, pH 8.4, andtert-butylmethylether (three times 0.7 ml). The aqueous phase containing polar compounds was neutralized with 100 mM HCl, and an aliquot was mixed with an equal volume of 200 mM sodium citrate buffer, pH 4, and incubated for 8 h at 37°C for hydrolysis of tertiary N-glucuronides. For deconjugation of the quaternary clozapine N+ -glucuronide, another aliquot was incubated for 2 h with 0.2 ml of 0.2 M sodium phosphate buffer, pH 7.0, and 0.1 ml of an aqueous 5% solution of β-glucuronidase (corresponding to 2000 Fishman units). All incubated samples were alkalinized with 0.1 ml of 25% ammonia and extracted three times with 0.7 ml of tert-butylmethylether. The combined organic phases were extracted with 0.1 or 0.2 ml of 50 mM sulfuric acid, an aliquot of which was injected for HPLC in system 1. Additional aliquots of the aqueous phase containing polar compounds were incubated at pH 7 for 2 or 8 h, respectively, and served as controls, with the small clozapine or desmethylclozapine quantities measured in them being subtracted from those in hydrolyzed samples. Recovery experiments were carried out by adding about 1.5 nmol of one of the N-glucuronides to 10 ml of urine from drug-free volunteers. The samples were processed in the same way as those from patients in parallel or along with reference samples ofN-glucuronides in which the contents of the conjugates were measured without initial solid-phase extraction. Reference solutions of tertiary N-glucuronides were initially extracted withtert-butylmethylether at alkaline pH to remove unconjugated compounds originating from spontaneous hydrolysis upon storage. Recoveries were 93 to 102% (mean 97%) for clozapine 5-N-glucuronide, 88 to 107% (mean 98%) for its desmethyl analog, and 93 to 98% (mean 96%) for clozapineN+ -glucuronide (n = 3–4). Due to the imprecision of standardization by UV spectrometry and to the lability of the tertiary N-glucuronides, data measured in urine have to be regarded as semiquantitative with an error up to 20%.
Enzymatic and Acid Hydrolysis.
The pH stability of clozapine 5-N-glucuronide was investigated by incubating 5 μM solutions in buffers composed of 20 mM each of acetic acid, MES, potassium dihydrogenphosphate, Tris, and glycine and adjusted to pH 4.5 to 7 with HCl or NaOH. Aliquots were drawn after 1 to 28 h and directly injected for HPLC analysis in system 2.
For enzymatic degradation, aqueous solutions of 1.5 to 2 nmol clozapine 5-N-glucuronide or clozapineN+ -glucuronide were incubated with about 2000 Fishman units/ml of β-glucuronidase from H. pomatia, pH 6 or 7, in a total volume of 0.24 to 0.7 ml, aliquots being drawn after 1 to 4 h. Analogous experiments were performed with 2 U/0.5 ml of β-glucuronidase from E. coli, pH 7, within up to 8 h. The aliquots of 0.1 to 0.2 ml were alkalinized with 0.05 ml of 2 N ammonia and twice extracted with 0.7 ml of tert-butylmethylether. The residue of the organic phases was dissolved in 0.1 ml of eluent for HPLC system 2.
HPLC Analyses.
System 1 comprised a 250- × 4.6-mm column with C18-silica gel (Prodigy 5 μm ODS; Phenomenex, Hösbach, Germany), the eluate being monitored at 290 nm and data being registered by the MT2 integration program (Kontron, München, Germany). The eluent was 50 mM ammonium acetate/acetonitrile (80:20, v/v) 1 ml/min for clozapine 5-N-glucuronide (k′, 8.1;RT, 20 min) and desmethylclozapine 5-N-glucuronide (k′, 3.2;RT, 9.3 min). The quantitation of clozapine (k′, 11.3; RT, 23.3 min) and desmethylclozapine (k′, 7.9; RT, 17 min) was based on peak areas and performed with 10 mM perchloric acid adjusted to pH 2.5 with NaOH/acetonitrile (72:28, v/v) 1 ml/min as the eluent.
In system 2, a 200- × 4.6-mm column filled with C18-silica gel 5 μm (Nucleosil 5 C18; Macherey-Nagel) was run with 0.02 M ammonium acetate in 0.9 M acetic acid (pH 3.0)/methanol (50:50, v/v) at 1 ml/min. The absorption of the eluate was measured at 290 nm, and peak heights served for quantitation of clozapine 5-N-glucuronide (k′, 2.3; RT, 7.5 min) and clozapine (k′, 4.2; RT, 11.8 min). Desmethylclozapine and its N-glucuronide hadk′ values of 3.1 and 1.9 (RT, 9.3 and 6.5 min), respectively.
Mass Spectrometry.
A TSQ 700 triple quadrupole mass spectrometer (Finnigan MAT GmbH, Bremen, Germany) and Finnigan acquisition software were used for spectra in the electrospray ionization (ESI) and collision-induced dissociation (CID) modes. The samples were dissolved in methanol/water (9:1) to concentrations of 10 to 20 ng/μl and infused into the ion source via a syringe pump at a flow rate of 1.5 μl/min. The electrospray needle voltage was +4500 V. The temperature of the heated transfer capillary was set to 120°C. Sheath gas was nitrogen. Spectra were acquired over the mass range 100 to 800 amu in 2 s during an acquisition time of 1 min. In the CID mass spectrometry mode, argon was used as collision gas. The collision cell pressure was 1.9 to 2.1 mtorr, and the collision offset voltage was −29 eV. The scan range was 20 to 510 amu, the scan time 1.5 s, and the acquisition time 2 min. The recorded spectra were averaged.
NMR Spectroscopy.
The 400-MHz 1H NMR spectra were recorded on a Bruker DRX 400 with a 5-mm TXI probehead at 303°K using Bruker standard software (Bruker, Newark, DE). The 1H data were referenced to a trace of tetramethylsilane (0.00 ppm). Samples were dissolved in deuterated methanol with 99.8% D. For processing of recorded spectra, the interferogram of the free induction decay with 32,000 data points was multiplied with a line broadening of −0.2 Hz.
Results
When human liver microsomes were incubated with 0.5 mM clozapine for 1 h, about 1% was converted to the quaternary ammonium glucuronide and about 4% to a metabolite presumed to be the 5-N-glucuronide. Desmethylclozapine was conjugated by about 1%. The UV spectra of all N-glucuronides in methanol resembled those of clozapine in water or methanol. Therefore, an alteration of the chromophore by substitution of the tertiary N-10 in the diazepine ring was not probable.
Distinct differences were apparent between the fragmentation patterns in CID mass spectrometry of clozapine 5-N-glucuronide and clozapine N+ -glucuronide (Fig.1). In the latter, [M + H]+ with m/z 503 for the35Cl isotope showed the four parallel fragmentations described previously (Schaber et al., 2001), which involve a loss of 100 amu (N-methylpiperazine) that must be preceded by an intramolecular rearrangement. A degradation of the piperazine ring by a loss of 57 amu took place from the base ionm/z 327 (clozapine) only but not from the protonated molecular ion. In contrast, such a degradation did occur with clozapine 5-N-glucuronide, resulting inm/z 446 in parallel to eliminations of two H2O resulting in m/z 485 and 467, of 92, 134 (fragmentation processes of the glucuronosyl residue), and 176 amu (glucuronic acid − H2O). Identical ESI-MS and MS/MS spectra were obtained with the tertiary glucuronides isolated from microsomal incubates and from patient urine (Fig. 1).
Desmethylclozapine 5-N-glucuronide from microsomes showed [M + H]+ 489, which in MS/MS lost two H2O, 92, 134, and 176 amu, as did the clozapine analog. The ESI-MS and MS/MS spectra of the compounds produced by microsomes and excreted by a patient were identical (Fig.2).
In 1H NMR (Table 1), the axial and equatorial protons in the piperazine ring of clozapine exhibited broad signals around 2.54 ppm (H-13 and H-14) and 3.43 ppm (H-12 and H-15) (Schaber, 1998). This is indicative of rapid equilibration of different chair forms of the piperazine ring. In contrast, one of these conformations is fixed in clozapine N+ -glucuronide, which can be concluded from the signals of equatorial protons (H-13 and H-14) at 4.14 ppm (triplet, J = 9.5 Hz; broad, 1 H) and 3.96 ppm (multiplet, broad, superimposed, 2 H, including one H-13/14ax). The aromatic protons of clozapineN+ -glucuronide were minimally influenced by the glucuronosyl residue, and no basic N-CH3group was detectable. The HH rotating frame nuclear Overhauser enhancement spectroscopy spectrum showed coupling of the anomeric proton H-1′ of the glucuronosyl group with other glucuronide protons and with those of the piperazine ring, but none with aromatic protons.
In clozapine 5-N-glucuronide, the piperazine ring protons H-13 and H-14 formed two broad singlets at 2.52 and 2.62 ppm, whereas H-12 and H-15 were probably present at 3.47 and 3.57 ppm, but with superposition. Of the glucuronosyl protons, only H-1′ could be assigned to a doublet at 4.61 ppm (J = 8 Hz) and a broad singlet at 4.52 ppm (integrated intensities together corresponding to 1 H). The other signals were extremely broad between 3.35 and 3.85 ppm. The signals of H-4 and H-6 were shifted down-field by 0.8 and 1.0 ppm, respectively, relative to those in clozapine. Together with the unchanged signals of a basic N-CH3 group at 2.35 ppm and those of the CH2 groups in the piperazine ring, this indicates that the zwitterion is probably protonated at N-10 with the possibility of mesomeric structures carrying a positive charge at N-5 (Fig. 3). The resonances of all aromatic protons were broadened, pointing to relatively slow inversion of the seven-membered ring. Consequently, signals generated by the glucuronosyl protons stem from at least three conformers and those of the piperazine ring protons from two times two conformers. The structures confirmed for the 5-N-glucuronides of clozapine and desmethylclozapine are shown in Fig. 3.
When clozapine N+ -glucuronide was incubated with β-glucuronidase from E. coli at pH 7, the liberation of clozapine was completed within 2 h, and the quantity corresponded to that expected on the basis of UV photometry. The same applied upon incubation with the enzyme fromH. pomatia for 1 or 2 h at pH 6 or 7. In contrast, no clozapine was liberated from clozapine 5-N-glucuronide by E. coliβ-glucuronidase at pH 7 within 2 and 4 h, and deconjugation with β-glucuronidase from H. pomatia amounted to 1% within 2 h. The acid hydrolysis rate of clozapine 5-N-glucuronide exhibited a steep increase between pH values of 6 and 4.5 (Fig. 4). Although substrate loss at pH 7 amounted to less than 10% within 28 h, it was 33% at pH 6 in the same time and 63 and 92% within 8 h at pH 5 and 4.5, respectively. Correspondingly, estimated half-lives varied from 190 h at pH 7 to 2 h at pH 4.5. In the latter case, a similar half-life (1.6 h) resulted for the appearance of clozapine in the incubate. The hydrolysis of desmethylclozapine 5-N-glucuronide was measured at pH 4.5 only; the conjugate disappeared with a half-life of 2.4 h, and the aglycone concentration increased with a half-life of 2.1 h.
In urine samples from four patients under clozapine monotherapy, the three N-glucuronides were assayed by solid-phase extraction, separation from unpolar compounds, and enzymatic or acid hydrolysis, respectively, followed by HPLC. In each one of the samples, all three conjugates were present, although their sum only accounted for about 0.36 to 1.3% of the clozapine dose (Table2). The lowest percentages of 5-N-glucuronides occurred in the two samples with pH 6.0, whereas higher values were measured in samples with pH values of 6.9 and 7.35.
Discussion
In the present investigation, the structure of the major clozapine conjugate produced in human liver microsomes in the presence of UDP-glucuronate was shown to be that of the 5-N-glucuronide. It can be supposed to be identical with “clozapine metabolite I” formed on incubation with expressed UDP-glucuronosyltransferase 1A4 (Green and Tephly, 1996). This enzyme concomitantly produced clozapine N+-glucuronide at about a 5-fold lower rate in agreement with the present findings in liver microsomes. Green and Tephly had also observed glucuronidation of desmethylclozapine, and this could now be demonstrated to occur at N-5 of the seven-membered ring. None of the tertiary N-glucuronides had previously been detected in human urine. In the investigation by Schaber et al. (2001), this was due to the occurrence of acidic conditions in the work-up procedure, which lead to rapid hydrolysis of the 5-N-glucuronides. For an identification by a single HPLC separation (Dain et al., 1997), excreted quantities are probably too small. In contrast, the most abundant metabolite of olanzapine in the urine and feces of volunteers given a single dose was the 10-N-glucuronide, which corresponds to clozapine 5-N-glucuronide. Its formation was estimated to account for 21 to 25% of the dose, with smaller quantities appearing as the quaternary N+ -glucuronide (Kassahun et al., 1997). This difference between the two structurally related drugs may be due to the predominance of oxidative attack in clozapine at the chlorine-substituted aromatic ring (Stock et al., 1977; Dain et al., 1997; Schaber et al., 2001) that is missing in olanzapine. Alternatively, the structure of olanzapine is favorable for glucuronidation at the secondary nitrogen of the central seven-membered ring. The two drugs are examples for regioselectiveN-glucuronidation reactions with tertiary and quaternary conjugates being produced in parallel in humans. The first observations on regioselectivity in N-glucuronide formation were made when substituted triazoles were incubated with human liver microsomes, and isomeric tertiary N-glucuronides were detected (Huskey et al., 1994).
The tertiary N-glucuronides of clozapine and olanzapine not only differ by their quantities excreted but apparently also by their acid stability. Incubation of plasma with an equal volume of 1 or 2 N HCl for 1 h at 50°C was required for 60 to 75% hydrolysis of olanzapine 10-N-glucuronide, whereas the corresponding clozapine glucuronide was decomposed to the same degree within 3 h at pH 4.5 and 37°C. This lability toward acidic conditions may be one of the reasons for the low percentage of the clozapine dose represented by urinary 5-N-glucuronide, namely 0.1 to 0.5% of the dose, the highest values being found in urine samples with higher pH values. The N+ -glucuronide, which was formed in vitro at markedly lower rates, represented 0.15 to 0.32% of the dose in urine, and an amount of 3% of the dose was reported for feces (Dain et al., 1997). In view of the higher formation rate of the tertiaryN-glucuronide in vitro, one would have expected higher excreted quantities, but these were not found. Discrepancies between relative quantities formed in vitro and determined in urine were also observed with regard to desmethylclozapine 5-N-glucuronide. Its urinary excretion was at least as high as that of clozapine 5-N-glucuronide, whereas its biosynthesis was much slower and its acid lability very similar.
Few examples of tertiary N-glucuronide formation from other secondary aromatic amines have been published (Chiu and Huskey, 1998). One of these is the formation of a pimobendan glucuronide, which in contrast to that of clozapine was not detected in vitro, but was among the major metabolites in human urine (Pahernik et al., 1995). Although data on the stability of the tertiary N-glucuronides (except those derived from hydroxylamines) are lacking, conjugates of primary aromatic amines are known to be very acid-labile (Green and Tephly, 1998). Glucuronidation principally is a reversible reaction in vivo, and this applies to quaternary N-glucuronides, too (Breyer-Pfaff et al., 1990). Because of their chemical stability (Mey et al., 1999; Kowalczyk et al., 2000), enzymatic hydrolysis must be the main factor. In contrast, olanzapine 10-N-glucuronide proved to be resistant toward β-glucuronidase from either E. coli or H. pomatia (Kassahun et al., 1997), and the same was observed with clozapine 5-N-glucuronide. Unless a β-glucuronidase with different substrate specificity is operative in humans, losses are probably due to the acid lability of this conjugate. These may result from uptake into intracellular compartments with low pH or following glomerular filtration when urine is acidified. The majority of clozapine liberated in kidney tubules will be reabsorbed (Schaber et al., 1998) such that formation of the tertiary N-glucuronide may initiate a futile cycle. On the other hand, since desmethylclozapine is in balance not reabsorbed, filtration of its 5-N-glucuronide and decomposition in tubular fluid will augment the apparent tubular secretion of desmethylclozapine (Schaber et al., 1998).
In conclusion, structural proof was obtained for tertiaryN-glucuronides of clozapine and desmethylclozapine, and it was demonstrated that, besides being synthesized in human liver microsomes, they were excreted by patients receiving clozapine. Estimation in urine was achieved by measuring aglycones liberated on acid hydrolysis of polar fractions. Acid lability steeply increased between pH values 7 and 4.5 and probably was a reason for the small percentage (0.2–1%) of the clozapine doses found in the form of tertiary N-glucuronides in patient urine. Quantities ofN-glucuronides in urine do not always reflect their formation rates in liver microsomes.
Acknowledgments
We thank Dr. I. Gaertner, Department of Psychiatry, University Clinic of Tuebingen, for providing patient urine samples. We are grateful to M. Cavegn, E. Endris, and U. Fischer (Boehringer Ingelheim, Biberach) for measuring NMR and mass spectra and to Dr. A. Ding and Dr. K. Wagner for the opportunity to use the analytical instruments.
Footnotes
- Abbreviations used are::
- HPLC
- high-pressure liquid chromatography
- MES
- 4-morpholineethanesulfonic acid
- ESI
- electrospray ionization
- CID
- collision-induced dissociation
- amu
- atomic mass unit
- MS
- mass spectroscopy
- Received April 11, 2001.
- Accepted June 29, 2001.
- The American Society for Pharmacology and Experimental Therapeutics