Abstract
The flavin-containing monooxygenases (FMOs) are important for the metabolism of numerous therapeutics and toxicants. Six mammalian FMO genes (FMO1–6) have been identified, each exhibiting developmental and tissue- and species-specific expression patterns. Previous studies demonstrated that human hepatic FMO1 is restricted to the fetus whereas FMO3 is the major adult isoform. These studies failed to describe temporal expression patterns, the precise timing of the FMO1/FMO3 switch, or potential control mechanisms. To address these questions, FMO1 and FMO3 were quantified in microsomal fractions from 240 human liver samples representing ages from 8 wk gestation to 18 y using Western blotting. FMO1 expression was highest in the embryo (8–15 wk gestation; 7.8 ± 5.3 pmol/mg protein). Low levels of FMO3 expression also were detectable in the embryo, but not in the fetus. FMO1 suppression occurred within 3 d postpartum in a process tightly coupled to birth, but not gestational age. The onset of FMO3 expression was highly variable, with most individuals failing to express this isoform during the neonatal period. FMO3 was detectable in most individuals by 1-2 y of age and was expressed at intermediate levels until 11 y (12.7 ± 8.0 pmol/mg protein). These data suggest that birth is necessary, but not sufficient for the onset of FMO3 expression. A gender-independent increase in FMO3 expression was observed from 11 to 18 y of age (26.9 ± 8.6 pmol/mg protein). Finally, 2- to 20-fold interindividual variation in FMO1 and FMO3 protein levels were observed, depending on the age bracket.
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Main
The FMOs (EC 1.14.13.8) are important for the NADPH-dependent oxidative metabolism of a wide variety of compounds containing nucleophilic nitrogen-, sulfur-, selenium-, and phosphorous-heteroatoms (1–4). Examples of known substrates of relevance to pediatric therapeutics include the antipsychotic chlorpromazine (5), the antihistaminics promethazine (6) and brompheniramine (7), the H2-receptor antagonists cimetidine (8) and ranitidine (9), and the gastroprokinetic agent itopride (10). However, given the prevalence of nitrogen- and sulfur-heteroatoms in medicinals, this short list is likely a gross underestimate of FMO's contribution to pediatric drug disposition. Environmental agents of particular concern include several thioether-containing organophosphorous pesticides (11), the carcinogen 2-aminofluorene (12), and the neurotoxicants nicotine (13) and 1-methyl-4-phenyl-1,2,3,6-tetrahydropyridine (MPTP) (14). Finally, a few dietary and/or endogenous FMO substrates have been identified, including trimethylamine, a break-down product of dietary choline (15), cysteamine (16), methionine, and several cysteine-S-conjugates (3).
Unlike the numerous cytochrome P450-dependent monooxygenases, there are only six mammalian FMO enzymes, each encoded by a distinct gene located on the long arm of human chromosome 1 (17, 18). As such, the FMO are considered more versatile with regard to substrate specificity than the cytochrome P450-dependent monooxygenases, a feature partly attributable to the FMO's unique catalytic mechanism (19). FMO species- and tissue-dependent expression has been well documented (20–23) and within a given species and tissue, gender- (24) and ontogenic-associated factors (23–25) also may affect FMO expression. Finally, genetic variability within the FMO locus also influences expression (26–29).
Several studies have documented significant changes in the expression of xenobiotic metabolizing enzymes during development (30–33). FMO1 is the major hepatic isoform in most mammals examined to date (4), with the exceptions of the adult human (34) and the adult female mouse (24) where FMO3 is the predominant isoform. FMO1 is expressed at relatively high levels in human fetal liver (23, 25) and also represents the major FMO enzyme in the adult human and rabbit intestine and kidney (22, 25). Thus, human FMO1 and FMO3 are subject to developmental and tissue-specific regulation, with a temporal switch in the hepatic expression of the two genes occurring some time after birth (23). However, the precise timing of these events and the control mechanisms remain unclear. Such knowledge would provide an improved ability to predict the selective morbidity of numerous toxicants and the efficacy of therapeutic entities, thus advancing our understanding of childhood susceptibility to chemical exposure and our ability to assess risk.
A goal of the current study was to gain a better understanding of the developmental expression pattern for human hepatic FMO1 and FMO3, including the definition of and potential variability in the temporal switch between the two enzymes. A second objective was to determine overall interindividual variation in FMO1 and FMO3 expression as a function of age.
METHODS
Materials.
Polyclonal antibodies raised against human FMO1 and FMO3 peptides and horseradish peroxidase-conjugated goat anti-rabbit IgG were obtained from GENTEST (Woburn, MA, U.S.A.). Protein molecular weight standards (bench mark prestained protein ladder) were from Invitrogen (Carlsbad, CA, U.S.A.). Nitrocellulose membranes and enhanced chemiluminescence Western blotting kits were purchased from Amersham Pharmacia Biotech (Arlington Heights, IL, U.S.A.). The micro bicinchoninic acid protein assay reagent kit was from Pierce Chemical (Rockford, IL, U.S.A.). All other reagents were obtained from common commercial sources at the purest grade available.
Tissue samples.
Frozen specimens of human liver were obtained from the Brain and Tissue Bank for Developmental Disorders, University of Baltimore and University of Miami (National Institute of Child Health and Human Development contract N01-HD-8–3284). Additional fetal and embryonic tissues were procured from the Central Laboratory for Human Embryology at the University of Washington. A total of 240 liver samples were obtained representing ages from 8 wk of gestation to 18 y of life. Gender information was provided for 221 samples, 137 being male and 84 female. Other than major diseases and cause of death, no other sample identifiers were available. Samples from individuals with disease processes that potentially would involve liver damage were excluded from the study. Tissue was stored at −80°C until used for the preparation of microsomal suspensions. This study was approved by the Children's Hospital of Wisconsin and the Medical College of Wisconsin Institutional Review Boards.
Preparation of microsomes.
Liver microsomes were prepared by differential centrifugation as previously described (35, 36) with some minor modifications. The frozen tissue was allowed to thaw at 4°C in homogenizing buffer containing 100 mM Tris-HCl, pH 7.4, 250 mM sucrose, 5 mM EDTA, 0.1 mM DTT, and 0.25 mM phenylmethylsulfonyl fluoride. After differential centrifugation, the microsomal pellet was resuspended in 100 mM potassium phosphate (pH 7.4) containing 1 mM EDTA and 0.15 M potassium chloride and centrifuged again at 104,000 ×g for 60 min. The pellet was resuspended in 100 mM potassium phosphate, pH 7.4, 1 mM EDTA, and 20% (vol/vol) glycerol, and stored in aliquots at −80°C. Protein concentrations were determined by the micro bicinchoninic acid protein assay (37) using BSA as a protein standard.
Electrophoresis and immunoblotting.
SDS-PAGE, using 10% resolving gels and a Tris-glycine running buffer, was performed according to the method of Laemmli (38). Fractionation was carried out using the Criterion Precast Gel Electrophoresis System (Bio-Rad, Hercules, CA, U.S.A.), followed by electrophoretic transfer to a nitrocellulose membrane using the Criterion Blotter (Bio-Rad) (39). Twenty micrograms of microsomal protein were used for each sample. Nonspecific binding sites were blocked by overnight incubation at 4°C with 5% nonfat dry milk in Tris-buffered saline (TBS; 25 mM Tris, pH 7.5, 150 mM sodium chloride). The blots were then incubated for 1 h at room temperature with FMO1 or FMO3 primary antibody diluted 1:5000 in TBS containing 0.5% nonfat dry milk. After extensive washing with several changes of TBS supplemented with 0.1% Tween-20, the blots were incubated for 1 h at room temperature with horseradish-conjugated goat anti-rabbit IgG diluted 1:10,000 in TBS containing 0.5% nonfat dry milk. Blots were then washed with several changes of TBS supplemented with 0.1% Tween-20 and processed for detection by enhanced chemiluminescence according to the manufacturer's instructions. The luminescence produced was detected by exposure of Fuji Super RX film (Fisher Scientific, Pittsburgh, PA, U.S.A.) and after digitizing the image using a Hewlett Packard 6300C scanner (Boise, ID, U.S.A.), the integrated OD of immunoreactive protein bands was determined using a Kodak DC120 digital camera and Digital Science 1D V 3.0 software (New Haven, CT, U.S.A.). Human FMO1 and FMO3 were expressed in a baculovirus vector expression system and insect cell membranes prepared as described previously (25). To quantify the amount of FMO in the preparations, the flavin adenine dinucleotide content of the membrane preparations was determined by HPLC (15). For a standard curve, membrane protein preparations representing 25, 50, 100, 250, and 500 fmol of FMO1 and FMO3 were included on each blot. The FMO1- and FMO3-specific content of the patient samples was determined by linear regression based on this standard curve (GraphPad Instat version 3.00, GraphPad Software, San Diego, CA, U.S.A.). The sensitivity limit was 0.2 fmol of FMO1 or FMO3. In all blots, bands corresponding to the protein of interest (FMO1 or FMO3) were identified by reference to the baculovirus-expressed FMO1 and FMO3 and molecular weight standards.
Data analysis.
Data breakpoints giving the maximum variance between groups and the least deviance within groups were determined by regression tree analysis using S-Plus 2000, a statistical package from Insightful Corp. (Seattle, WA, U.S.A.). Samples with specific contents falling at least 1.5 times outside the 25th to 75th percentile values were considered outliers and were not included in the analysis. The significance of differences between groups was confirmed by a Kruskal-Wallis nonparametric analysis of variance with Mann-Whitney U tests used for pair-wise comparisons. Multiple comparisons were corrected for using a Bonferroni adjustment (the p value multiplied by 3). A p value < 0.05 was accepted as significant.
RESULTS
Developmental expression pattern for FMO1 and FMO3.
Previous studies provided evidence for FMO1 and FMO3 differential expression in human liver during development (40, 23, 25). However, none of these reports addressed the temporal expression pattern of these enzymes, the precise timing of the FMO1/FMO3 switch, or potential control mechanisms. In the present study, the developmental expression pattern of human hepatic FMO1 and FMO3 was determined by SDS-PAGE and Western blot analysis of microsomal protein prepared from a bank of 240 human liver samples. Western blotting with antibodies to FMO1 or FMO3 revealed immunoreactive bands with apparent molecular masses near 60 kD, corresponding to full-length FMO1 or FMO3, respectively. Figure 1, A and B, depicts representative blots with human hepatic microsomes of different ages. No cross-reactivity was observed between the respective antibodies and antigens, even at the highest protein levels used (500 fmol). In agreement with previous studies, FMO1 expression was present in embryonic and fetal liver (Fig. 1A) but not in any of the postnatal liver samples. In contrast, FMO3 expression was not detectable in fetal liver samples, but was present in postnatal samples (Fig. 1B). The coefficient of determination (r2) values for the standard curves ranged from 0.960 to 0.998 (median = 0.990) and typical coefficients of variation for independent experiments were 5.6 for FMO1 (n = 5) and 4.6 for FMO3 (n = 6).
The overall developmental-specific expression patterns for FMO1 and FMO3 are shown in Figure 2, A and B. Although there was significant interindividual variation, the highest level of FMO1 expression was observed at the earliest gestational ages, i.e. less than 15 wk (Fig. 2A). After this period, there was a decline in FMO1 expression up to 40 wk (term). In contrast to earlier reports (40, 23), low levels of FMO3 expression were detected in 7 of 38 embryonic samples between 8 and 15 wk gestation (1.4 ± 0.9 pmol/mg microsomal protein). No FMO3 expression was observed between 15 and 40 wk gestation. The FMO1/FMO3 developmental expression pattern was quite different after birth. As shown in Figure 2B, there was a dramatic decline in FMO1 expression within the first few days of life. Although variable, the onset of FMO3 expression was generally observed during the first year of life followed by moderate expression up to 11 y of age. Significant interindividual variability also was observed during this period. A second phase of FMO3 expression was observed from puberty to adult, where FMO3 expression increased to a maximum level of approximately 40 pmol/mg microsomal protein. No correlation was observed between FMO1- or FMO3-specific content and the postmortem interval, i.e. the time between death and the freezing of liver tissue (data not shown).
Definition of the FMO1/FMO3 temporal switch.
To better elucidate the precise timing of the hepatic FMO1/FMO3 isoform switch, an expanded plot of FMO1 and FMO3 expression during the neonatal period (birth to 30 d) and the first year of life was examined (Fig. 3). FMO1 expression was low, but detectable in most samples within the first 3 d of life, but then was extinguished in all but a few samples. In contrast, the onset of FMO3 expression was highly variable during the neonatal period and, when present, was low relative to expression levels observed at later ages. A significant increase in expression was observed between the neonatal period and 1 y of age. As a first approach to determining the mechanism(s) regulating the FMO1/FMO3 isoform switch, an analysis of specific FMO content as a function of gestational and postnatal age was performed using liver samples from premature infants that lived for a defined period of time after birth (Fig. 4). From this analysis, FMO1 expression clearly was extinguished within the first few days of life, irrespective of gestational age, consistent with the suppression of FMO1 expression being tightly linked to the birth process, but not maturity. A direct linkage of birth to the onset of FMO3 expression was less clear. With the exception of 4 outliers from a total of 15 samples, FMO3 expression was nondetectable during the first 3 d of life, irrespective of gestational age. From Figure 2A, no FMO3 expression was detectable in any of the late fetal samples that did not survive for any defined period after birth. Low but detectable FMO3 expression was observed in 4 of 13 samples between 4 d and 30 wk postnatal age, irrespective of gestational age at the time of birth. Together with the results presented in Figure 3, these data are consistent with birth being necessary but not sufficient for the onset of FMO3 expression.
Interindividual and temporal variation in FMO1 and FMO3 expression.
To better summarize the different phases of FMO1 and FMO3 developmental expression, as well as quantify the interindividual variability in expression, the data presented in Figures 2–4 were re-analyzed using regression trees. This method determined data breakpoints that would provide for maximal variation in data between groups and minimal deviation within a group. Results of this analysis are shown in Figure 5. From this analysis of the data, FMO1 expression divides into three phases approximately matching the trimesters of development. Maximum FMO expression was observed in samples <15 wk gestation (7.8 ± 5.3 pmol/mg microsomal protein). During the second trimester (15 wk to 6 mo), mean expression levels decreased by approximately 50% (3.8 ± 2.6 pmol/mg microsomal protein) and again by a further 50% (2.1 ± 1.8 pmol/mg microsomal protein) in the third trimester. FMO1 expression was essentially nondetectable after 3 d postpartum. Interindividual variation in FMO1 expression during the prenatal period was 10- to 20-fold. FMO3 expression was only observed in a small number of samples and only during the embryonic period at <15 wk gestation (see Fig. 2A). After 2–3 d postpartum, overall FMO expression (FMO1 plus FMO3) was absent in the majority of samples and remained low to nondetectable for the first 3 wk of life. In those with detectable protein, FMO3 predominated with expression levels that were <5% of those observed in the adult (1.1 ± 3.3 pmol/mg microsomal protein). The regression tree analysis suggests that the postneonatal FMO3 expression can be divided into three phases. Between 3 wk and 10 mo, mean FMO3 expression increased 5-fold (4.7 ± 5.9 pmol/mg microsomal protein) and then another approximate 3-fold between 10 mo and 11 y (12.7 ± 8.0 pmol/mg microsomal protein). Between 11 and 18 y of life, there was a third significant increase in mean expression levels (2-fold increase to 26.9 ± 8.6 pmol/mg microsomal protein). Pair-wise comparisons of FMO1- and FMO3-specific content between each of the age brackets demonstrated significant differences between all age brackets (p < 0.05).
Gender-selective FMO expression.
Given the previous studies indicating the ability of the sex steroids and/or gender to modulate FMO expression in animal models (24, 41–45) and the evident increase in FMO3 expression at puberty in the current study, the potential role of gender in regulating postnatal human hepatic FMO expression was examined. When gender was entered as a possible categorical variable in the regression tree analysis, it failed to enter into the model (data not shown). Thus, in the human, gender-associated factors do not appear important in either the pre- or postpuberty phases of FMO3 expression.
DISCUSSION
Previous studies provided evidence for FMO isoform switching in the human from FMO1 in fetal liver to FMO3 in the adult (23, 25). However, the precise timing of this event and specific control mechanism(s) remained unknown. Further, these previous studies were limited in scope to short windows of time during development and also by relatively small sample sizes. In the present study, an effort was made to comprehensively characterize the developmental expression pattern for human hepatic FMO1 and FMO3, better defining the temporal switch between the two enzymes and determining interindividual variation in expression. Western blot analysis of 240 human liver microsomal samples, ranging from 8 wk gestation to 18 y of life, confirmed that FMO1 is the major fetal isoform whereas FMO3 is the major adult isoform. The highest level of FMO1 expression was observed in embryonic samples at 8 to 15 wk gestation. In contrast to earlier reports (40, 23), low levels of FMO3 expression were detectable in some embryonic samples, but not in fetal samples. This discrepancy may be due to the low sample numbers used in previous studies, uncertainty about the age of these samples, and/or the sensitivity of the assay used. The results reported herein also suggest that FMO1 suppression occurs within the first few days of life in a process that is tightly coupled to birth, but not gestational age. However, FMO1 suppression is not directly linked to the onset of FMO3 expression (linear regression correlating FMO1- and FMO3-specific content during first year of life, r2 = 0.009) (data not shown). The latter is highly variable, with most individuals failing to express FMO3 during the neonatal period (first 30 d of life). When neonatal expression was detectable, it was 5 to 10% of adult levels, although one individual exhibited FMO3 protein levels approaching those seen in the adult. Thus, with rare exception, hepatic FMO expression is absent or low during the neonatal period in the human. This conclusion assumes the absence of other FMO isoforms, however, previous studies have suggested that FMO2, FMO4, and FMO5 are not expressed, or are expressed at very low levels in the human liver (46). Very little is known regarding FMO6 and, thus, the contribution of this enzyme remains a potential limitation to the interpretation of these data. FMO3 expression is detectable in most individuals by 1–2 y of age and is expressed at intermediate levels until approximately 11 y. Taken together with the absence of detectable fetal FMO3 protein, these results suggest that birth is necessary but not sufficient for the initial onset of FMO3 expression. A further increase in FMO3 expression is observed from 10 to 18 y of age, reaching a maximum level of approximately 40 pmol/mg microsomal protein in the current sample population. This level of FMO3 expression is not as high as the maximum reported by Overby et al.(47), but does fall within the range of values reported by these investigators (5–112 pmol/mg microsomal protein). It is possible that maximum adult levels have not been reached by the highest age represented in the current study, i.e. 18 y. Importantly, neither the onset of FMO3 expression nor the increase in expression at puberty appears linked to gender. Finally, FMO1 and FMO3 expression varies 2- to 20-fold among individuals, depending on the age bracket.
A few studies have reported FMO developmental expression patterns in experimental animal models, although most limited their studies to late fetal stages and postnatal development. In the rabbit lung, FMO2 expression was observed in the fetus and during the neonatal period, in some instances approaching levels observed in the adult animal (48). However, in the liver, FMO1 is a major isoform observed in the rabbit and most other mammalian species, and as such, it is difficult to extrapolate results from these models to the human. A possible exception is the mouse. Cherrington et al.(24) demonstrated the presence of substantial FMO1 and FMO5 expression in CD-1 mouse liver as early as 15 d gestation. However, FMO3 was nondetectable during any prenatal period. FMO3 was detectable in the CD-1 mouse liver by 2 wk postpartum. However, in contrast to what is observed in the human, hepatic FMO1 continues to be expressed postpartum in the mouse. Also in contrast to the human, substantial gender differences in hepatic FMO expression become apparent in the adult rodent models. Thus, FMO3 expression is suppressed in the adult male, but not female mouse and FMO1 expression also is significantly higher in the female versus male. FMO3 expression in the adult rat was gender-independent. Thus, the similarities between the animal models and the human appear restricted to the expression of FMO1 in the fetal liver and the onset of FMO3 expression shortly after birth. The absence of FMO1 suppression and the overall gender differences in FMO expression again cause one to question the validity of extrapolating data from these animal models to the human.
The observed FMO1 and FMO3 developmental expression pattern is somewhat reminiscent of the pattern observed for two human CYP3A isoforms. Similar to what is observed in the present study, CYP3A7, but not CYP3A4, is expressed at easily detectable levels in human embryonic hepatic tissues at 7–9 wk of gestation (49), as well as in later fetal stages of development (50). Maximal CYP3A7 activity is observed within the first week of life, but then slowly declines to nondetectable levels in the adult. In contrast, CYP3A4 expression is low or nondetectable in the fetal period, but is activated during the first week of life irrespective of gestational age. By 1 y, CYP3A4 expression is at a level approximately 50% of that seen in the adult (50). Although the temporal switch in CYP3A expression shows some similarity to that observed for FMO, important differences also are noted. First, in contrast to CYP3A4, FMO3 expression is nondetectable in the fetal liver. Second and perhaps more importantly, the suppression of CYP3A7 and activation of CYP3A4 appear directly linked such that overall CYP3A expression is essentially constant (50). In contrast, the suppression of FMO1 and the activation of FMO3 do not appear linked. FMO1 suppression occurs within the first 2 to 3 d of life whereas the onset of FMO3 expression does not occur in some individuals until 1–2 y. Thus, in contrast to CYP3A, overall FMO expression is low to nondetectable in the neonatal period. Given the differential ability of FMO1 and FMO3 to catalyze the oxidation of trimethylamine to its N-oxide (15), this observation likely explains the observation of trimethylaminuria in a 2-mo- and a 4-y-old patient that resolved with no intervention by 4 mo and 5 y, respectively (51). Finally, C/EBPα (CCAAT/enhancer-binding protein alpha) and DBP (D-element-binding protein) transcription factors have been implicated as controlling factors for the temporal CYP3A switch (52). Although a role for these factors in regulating the onset of FMO3 expression has not been examined, HNF1α and HNF4α have been shown to be the major transcription factors controlling the expression of rabbit and human FMO1, whereas C/EBPα does not appear to have a significant role (53). Taken together, these observations suggest very different mechanisms controlling the CYP3A and FMO temporal switches in the human.
Several studies have implicated a role for sex steroids and/or gender in regulating FMO expression in animal models. Testosterone has been shown to suppress FMO1 and FMO3 hepatic activity in the mouse, but stimulatory effects of 17β-estradiol were not observed (41, 44). These modulating effects of testosterone largely account for the hepatic FMO1 and FMO3 gender differences in this species. In contrast, 17β-estradiol has been shown to suppress FMO activity in rat hepatocytes (45), however, no gender-dependent FMO1 or FMO3 expression was observed in the livers of intact animals (12). Both progesterone and glucocorticoids have been implicated in stimulating FMO2 expression in the rabbit lung and kidney (54, 43), perhaps explaining some of the noted gender differences in FMO expression observed in this species (22). In marked contrast to results for each of these animal models, there is little or no evidence for steroid-regulation of human hepatic FMO expression (24). Consistent with this observation, neither the repression of FMO1 at birth, the onset of FMO3 expression at 1–2 y, or the increase in FMO3 expression at puberty were correlated with gender in the current study.
Significant interindividual variability in the expression of human FMO has been reported. Using monospecific antibodies, Overby et al.(47) reported a 10-fold variation in hepatic FMO3-specific content which, despite a limited sample size (n = 5), agrees favorably with several reports on activity measurements using specific substrates and preparations of human hepatic microsomes (55–57). A similar earlier study on fetal liver, also limited to a sample size of five, reported a 2-fold variation in FMO1 specific content (25). Most importantly, other than restricting their studies to fetal or adult samples, these reports failed to control for changes in FMO1 and FMO3 expression as a function of age. Based on the data reported herein, this is a major confounding factor in interpreting these earlier reports. In the current study, the much larger sample size allowed for stratification according to major age brackets between which significant differences in FMO expression were observed. In general, the results corroborate the earlier reports, providing confidence in the conclusion of considerable interindividual variability in both FMO1 and FMO3 expression. Within each age bracket and excluding samples in which no immunoreactive FMO was detectable as well as outliers, specific content varied from 2- to 20-fold. Dietary indoles are the only environmental substances known to modulate FMO expression, suppressing FMO3 levels 2- to 3-fold (58, 59). However, it is unknown whether indoles are able to similarly modulate FMO1 and further, it is unlikely that such dietary components would be responsible for the variability among the fetal and neonatal samples. Interindividual variation might also be explained by genetic differences. Although no polymorphisms have been reported for human FMO1, several genetic variants have been reported for human FMO3(26–28, 60–65). However, variants representing nonsense mutations that would be expected to affect FMO3 specific content are rare (62, 61). Thus, the variation observed in the present study most likely represents variation in factors controlling FMO1 and FMO3 expression and/or regulatory polymorphisms that remain to be elucidated.
In summary, this study describes the developmental expression pattern for human hepatic FMO1 and FMO3. The temporal switch between these two enzymes has been defined. Further, it is clear from these data that the variability in the switch is almost exclusively accounted for by variability in the onset of FMO3 expression. Considerable interindividual variation in FMO1 and FMO3 expression within each of the defined age brackets also has been confirmed, most likely because of variation in factors regulating expression. The relatively high levels of FMO1 expression observed throughout prenatal development and in particular during the embryonic periods cause one to question whether or not this enzyme might be playing some developmentally important function. However, a role for FMO, and, in particular, FMO1, in the metabolism of endogenous substances remains elusive. FMO1 has been implicated in the oxidation of methionine, cysteamine, and numerous cysteine-S-conjugates (3), but the significance of these pathways to development, if any, is not apparent. In contrast, the FMO are recognized as being important for the metabolic disposition of a wide variety of therapeutics and environmental toxicants. It is clear that isoform switching, changes in expression as a function of age, and interindividual variability in expression will have a significant impact on therapeutic efficacy and toxicant susceptibility. This particularly will be true for drugs with narrow therapeutic indices and toxicants that require metabolism for either detoxification and/or bioactivation. Although our knowledge concerning the molecular mechanisms controlling FMO expression remains deficient, the data reported in this study offer significant insight into the developmental expression pattern for both FMO1 and FMO3 that will be important for the elucidation of these regulatory mechanisms.
Abbreviations
- FMO:
-
flavin-containing monooxygenase
- TBS:
-
Tris-buffered saline
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Acknowledgements
The authors thank D. Gail McCarver, M.D., Department of Pediatrics, Division of Neonatology, Medical College of Wisconsin, for assistance in evaluating disease processes that might have resulted in damage to the available liver samples.
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Supported, in part, by National Institutes of Health Grants CA53106 (R.N.H.) and GM43511 (A.E.R.). C.K.Y. was supported by National Institutes of Health Training Grant GM07750.
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Koukouritaki, S., Simpson, P., Yeung, C. et al. Human Hepatic Flavin-Containing Monooxygenases 1 (FMO1) and 3 (FMO3) Developmental Expression. Pediatr Res 51, 236–243 (2002). https://doi.org/10.1203/00006450-200202000-00018
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DOI: https://doi.org/10.1203/00006450-200202000-00018
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