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Age-related changes in the mRNA levels of CYP1A1, CYP2B1/2 and CYP3A1 isoforms in rat small intestine

Abstract

It has been established beyond doubt that, as well as the liver, the small intestine is an important site of first-pass metabolism of numerous drugs, food components and toxic xenobiotics. However, there is not much information available about age-dependent changes of intestinal biotransformation pathways. In the present paper, we evaluated the relationships between intestinal cytochrome P450 complex activity and the age of animals. The study was carried out on male Sprague–Dawley rats (n = 5) from 5 age series: 0.5-, 2-, 4-, 20-, and 28 months old. Animals at every age series were divided into 4 groups: control and three groups of rats treated with the CYP450 specific inducers: phenobarbital, ÎČ-naphtoflavone and dexamethasone, respectively. RNA was isolated from intestinal mucosa, and then standard RT-PCR was used for the analysis of CYP1A1, CYP2B1/2 and CYP3A1 mRNA expression. Additionally, the activities of NADPH-cytochrome P450 and NADH-cytochrome b5 reductases in the microsomal fraction were biochemically estimated. The constitutive intestinal CYP1A1 mRNA expression changes during maturation and aging. Inducibility of CYP1A1 gene was evident in intestinal mucosa at 2-, 4- and 20-month-old rats. A similar pattern of changes was observed for CYP2B1/2 isoforms. CYP3A1 mRNA expression was not detected in small intestine of 2-week-old rats. In matured rats, constitutive intestinal CYP3A1 expression was low, although after induction, significant increases in CYP3A1 mRNA amount were noted in aged individuals. Intestinal activity of both analyzed reductases was lowest in immature rats and highest in 28-month-old animals. In conclusion, the activity of cytochrome P450 complex in rat small intestine was not decreased by the aging processes, so the high rate of oxidative metabolic reactions in intestinal mucosa can be maintained till the advanced life stage.

Introduction

Cytochrome P450-dependent metabolic pathways seem to play a crucial physiological role in all vertebrate species. The activity of this important system can be changed by inhibition or induction of the enzymes by the numerous drugs and other compounds that occur in the food, e.g., in fruits, herbs, vegetables as well as in either alcoholic or soft beverages (Ware 2009; Nekvindova and Anzenbacher 2007; Hidestrand et al. 2005; Fujita 2004). From the medical viewpoint, it is essential that these universally used substances do not cause failure of therapies causing serious health alterations. For example, potentially dangerous interactions of grapefruit or lemon juices, a potent cytochrome P450 inhibitors, with felodipine and cyclosporine, red wine with cyclosporine and St John’s wort with various medicines have been well demonstrated (Cuciureanu et al. 2010; Uesawa et al. 2010; Paine et al. 2008; Chaudhary and Willett 2006; Tsunoda et al. 2001; Baltes et al. 2001). Many potentially harmful food contaminants such as heterocyclic aromatic amines identified in fried meat, phenol complexes from the components of the Mediterranean diet and ethyl carbamate present in some kinds of brandy are able to induct some isoforms of cytochrome P450 in various organs (HĂŒmmerich et al. 2004; Stupans et al. 2001; Kleman et al. 1995; Guengerich et al. 1994). Although, the biotransformation of xenobiotics takes place mostly in the liver, some extrahepatic cytochrome P450 complexes (e.g., gastrointestinal, renal and pulmonary) contribute substantially to the total metabolic potential of the living mammals. The small intestine is one of the organs involved in cytochrome P450-dependent metabolism of various food-derived substances, drugs and toxic agents (Martignoni et al. 2006). Metabolic processes performed by the gut mucosa may affect uptake, efflux and transport of orally delivered pharmaceuticals and dietary xenobiotics by cells, tissues and organs (Benet et al. 2004; Zhang and Benet 2001; Watkins 1997). The CYP3A4-dependent interaction by food-derived agents may be related to the high level expression of CYP3A4 in the small intestine, as well as its broad substrate specificity (Fujita 2004). It has been confirmed that role of intestinal metabolism is significantly greater than hepatic in the first-pass effect for some drugs, e.g., cyclosporine A and midazolam (Isin and Guengerich 2007; Kanazu et al. 2005; Kotegawa et al. 2002; Paine et al. 1996). Even more than half a percent of orally administered cyclosporine A is metabolized by enterocytes (Hebert 1997). The intestinal mucosa, therefore, is considered one of the most important sites of drug metabolism. Numerous recent studies have demonstrated that the intestinal epithelium contributes to the biotransformation of diltiazem and nifedipine (Mitschke et al. 2008; Iwao et al. 2004). On the other hand, local activation of procarcinogens in the small and large bowel via cytochrome P450-dependent microsomal monooxygenase metabolic pathway is considered to be an important factor in cancer etiology. The CYP1A1 isoform shows the highest level of expression in rat small intestine (Zhang et al. 1999). The other CYP450 isoforms were found in the epithelium of rat small intestine include CYP1A2 (Hakkak and Ronis 1993), CYP2B, CYP2C, CYP2E1, CYP3A, (Perloff et al. 2004; Takemoto et al. 2003), CYP4A1 (Catterall et al. 2003), CYP4F12 (Stark et al. 2004), CYP2J4 and CYP2J3 (Zhang et al. 1998). The extended exposure to the ritonavir and dexamethasone increased the expression of CYP3A isoforms in rat enteric mucosal cells (Perloff et al. 2004). In the human small intestine, mRNAs of CYP1A1, CYP1B1, CYP2C, CYP2D6, CYP2E1, CYP3A4 and CYP3A5 were identified (Ding and Kaminsky 2003), but only CYP3A4, CYP3A5 and, on minimal level, CYP1A1 (Zhang et al. 1999) were detected as proteins. Both omeprazol and acetylsalicylic acid act as potent inducers of CYP2D6, CYP2E1, CYP3A4 (Lindell et al. 2003).

It should be emphasized that in human intestinal mucosa, the members of CYP3A family play the leading role, especially CYP3A4 isoform (Emoto et al. 2000), which participates in metabolism of many xenobiotics and drugs and is generally responsible for the biotransformation of more than 50% of clinical pharmaceuticals. Moreover, CYP3A4 appears to be a key enzyme in food–drug interactions (Fujita 2004). The content of CY3A4 isoform is most abundant in the proximal portion and is decreased distally in the human and rodent small intestine (Zhang et al. 1999, De Waziers et al. 1990). The members of CYP1, CYP2 and CYP3 families are also expressed in human and animal colon (Bernauer et al. 2002).

Morphological and biochemical differentiation, which takes place in mammalian intestinal tract during maturation and aging, seems to be strictly related to the development of cytochrome P450 complex, which also includes the specific reductases as well as donors of electrons for CYP450-dependent catalytic cycle. Nevertheless, most experiments that referred to cytochrome P450-dependent intestinal metabolism concerned young, sexually mature animals. The main purpose of this study was to analyze the relationships between intestinal expression of selected cytochrome P450 mRNAs (CYP1A1, CYP2B1/2, CYP3A1) and the age of rats. A further aim of our experiment was the evaluation of age-related changes in the activities of NADPH-cytochrome P450 and NADH-cytochrome b5 reductases. In the present study, we focused on investigating the changes in the mRNA expression of the main intestinal cytochrome P450 isoforms as well as on evaluating the nonspecific activity of the reductases mentioned above. We have not studied either metabolic activity or protein expression corresponding to any CYP isoform. The first results of our experiment concerning age-dependent changes of selected cytochrome P450 proteins in rat small intestine were previously reported (PaƂasz et al. 2003). The NADPH-cytochrome P450 and NADH-cytochrome b5 reductase activities presented in this article are not relating to CYP450 isoforms. Although the rate of biotransformation of the substrates to metabolic products was not measured, owing to that all the results reflects the CYPs activity merely indirectly, we suppose that the evaluation of age-related expression and inducibility of the intestinal CYP450 mRNAs and the activity of the reductases may also be helpful in the better understanding of intestinal metabolism. We appreciate the fact that our studies do not reflect the intestinal CYP450 activity in humans; nevertheless, any clinical equivalent of our experiment would be very difficult to perform.

Many carcinogenic metabolites are the products of CYP450-dependent microsomal activation of various food-derived substances such as aflatoxin B1 that is transformed to the genetically harmful exo-8,9-epoxide. Other food components affect the activity of selected CYP isoforms, e.g., flavones stimulate while naringenin, a major flavonoid of grapefruit juice, attenuates the rate of xenobiotic metabolism (Guengerich et al. 1994). Probably, the diet-related induction of the CYP genes in the small intestine of aged rats and humans could play an important role in cancer etiology within this organ. On account of that, the studies focusing on age-related changes of CYPs expression in the alimentary tract could also be interesting for scientists working in the field of nutrition and dietetics. Nevertheless, it should be clearly emphasized that the study reported herein may be value as an experimental paradigm to evaluate the cytochrome P450-dependent metabolism in animals. The clinical applicability of this model is extremely limited by numerous species differences in patterns of metabolic biotransformation as well as intestinal profile of CYP450 isoforms.

Materials and methods

Animals

The studies were carried out on 100 male Sprague–Dawley rats, and animals from 5 age series, 0.5-, 2-, 4-, 20-, and 28-month-old individuals, were divided into 4 experimental groups (n = 5): one control group and three groups of rats that were induced with selective CYP1A1, CYP2B1/2 and CYP3A1 inducers. The rats of all groups were fed on standard diet (Murigran, drinking water) and kept under the same conditions at 22°C with a regular 4-h day/night cycle. The induced groups of animals have received intraperitoneally two doses (for 2 consecutive days) of phenobarbital (50 mg/kg), ÎČ-naphtoflavone (80 mg/kg) or dexamethasone (30 mg/kg), respectively. It should be emphasized that the inducers used in this study are strictly appropriate to studied rat CYP450 isoforms, and they do not correspond to inducers of human enzymes. All the agents were administered at the same time when the rats were active, at approximately 7.00 AM to avoid any circadian changes. On the third day, the animals were quickly anaesthetized with halothane and then were killed immediately by decapitation. All experimental procedures were approved by local bioethic committee at the Medical University of Silesia.

RT-PCR

The small intestines were completely excised directly after sacrifice and then rinsed with cold phosphate buffer pH 7.3 containing 1.5 mM KCl and 96 mM NaCl. Total mRNA was extracted from manually scrapped 50 mg samples of intestinal mucosa (each sample was taken from one individual) using Trizol TM according to Chomczynski and Sacchi (1987), and then RT-PCR method was used to analyze CYP1A1, CYP2B1/2 and CYP3A1 mRNA expression. Collected RNA samples were transcribed into cDNA during incubation in buffered solution of reverse transcriptase MMLV-RT with RNAsin, oligo-dT and mix of nucleotides at 37°C for 90 min. using DNA Thermal Cycler 480 (Perkin Elmer Inc., Waltham, MA). The PCR was performed in Peltier Thermal Cycler PT-200 (MJ Research Inc., Watertown, MA) for 26 rounds; 1 min. at 94 °C 1 min. at 65°C (CYP1A1), 55.8°C (CYP2B1/2) or 62.3°C (CYP3A1) and finally 90 s. at 72°C. The studied mRNAs and standard internal reference glyceraldehyde phosphate dehydrogenase (GAPDH) mRNA were amplified using the following primers CYP1A1; forward: 5â€Č-GATGCTGAGGACCAGAAGACCGC, reverse: 5â€Č-CAGGAG GCTGGACGAGAATGC; CYP2B1/2; forward: 5â€Č-CCAAGCGCTCCACGAGACTT, reverse: 5â€Č-TTGGGAGCAGGTACCCTC, CYB3A1; forward: 5â€Č-CCGCCTGGATTCTGTGCAGA, reverse: 5â€Č-TGGGAGGTGCCTTATTGGGC, GAPDH; forward: 5â€Č-GTG AACGGATTTGGCCGTATCG, reverse: 5â€Č-ATCACGCCACAGCTTTCCAGAGG. Products of PCR amplification were separated on 2% agarose gel and visualized with ethidium bromide and then were photographed in UV light chamber. Semiquantitative densitometric analysis was performed with the use of OneDScan software (Scanalytics), and the results were expressed on graphs as integrated optical density (IOD).

Enzymatic assay

Microsomal fraction was prepared from the homogenates of intestinal mucosa (0.25 M sucrose in 100 mM phosphate buffer) by centrifugation (100,000×g, 90 min.) of the postmitochondrial supernatant (9,000×g, 20 min.) as previously described (Dallner 1974). Microsomes were resuspended in 20% buffered glycerol and stored at −80°C until analysis. The activities of NADPH-cytochrome P450 and NADH-cytochrome b5 reductases were estimated in microsomal fraction using NADH, NADPH and cytochrome c buffered solutions according to Hodges and Leonard method (1974). All the results were analyzed statistically by Student–Newman–Keuls test (P < 0.05).

Results

The results show clearly that mRNA expression of the studied intestinal CYP450 isoforms changes its function depending on age (Figs. 1, 2, 3; Tables 1, 2, 3). Constitutive expression of CYP1A1 mRNA was lowest in immature 2-week-old rats. Statistically significant increase in CYP1A1 mRNA expression in comparison with the immature animals was found in 4-, 20- (P < 0.001) and 28-month-old ones (P < 0.01). In sexually mature rats, the level of CYP1A1 mRNA was relatively stable till the advanced age. An increase in CYP1A1 mRNA expression was also observed in individuals treated with ÎČ-naphtoflavone. The highest CYP1A1 gene inducibility (increase in the amount of PCR product in induced groups in relation to control groups) was detected in 2-week-old animals (1998% of control) and the lowest in the 28-month-old ones (112% of control). Individuals at age of 2, 4, and 20 months showed similar CYP1A1 gene inducibility: 237, 284 and 266% of control, respectively.

Fig. 1
figure 1

Age-related constitutive and ÎČ-naphtoflavone-inducible expression of CYP1A1 mRNA in rat small intestine. Values are expressed as mean integrated optical density (IOD) ± S.D. Significant difference at **P < 0.01 and *P < 0.05 versus control immature 2-week-old rats, at † P < 0.05 versus control 2-month-old rats, at filled circle P < 0.05 versus control 4-month-old rats, at ## P < 0.001 and # P < 0.05 versus induced 2-week-old animals and at filled double diamond P < 0.01 and filled diamond P < 0.05 versus induced 2-month-old individuals

Fig. 2
figure 2

Age-related constitutive and phenobarbital-inducible expression of CYP2B1/2 mRNA in rat small intestine. Values are expressed as mean integrated optical density (IOD) ± S.D Significant difference at ***P < 0.001 and **P < 0.01 and *P < 0.05 versus control immature 2-week-old rats, at ‡ P < 0.01 and † P < 0.05 versus control 2-month-old rats, at filled circle P < 0.05 versus induced 2-week-old rats, at # P < 0.05 versus induced 2-month-old animals, at filled square P < 0.01 versus induced 4-month-old rats, at filled diamond P < 0.05 versus induced 20-month-old individuals

Fig. 3
figure 3

Age-related constitutive and dexamethasone-inducible expression of CYP3A1 mRNA in rat small intestine. Values are expressed as mean integrated optical density (IOD) ± S.D. Significant difference at *P < 0.05 versus control immature 2-week-old rats, at ‡ P < 0.01 and † P < 0.05 versus induced 2-week-old rats, at filled circle P < 0.05 versus induced 2-month-old rats, at filled square P < 0.05 versus induced 4-month-old rats, at filled diamond P < 0.05 versus induced 20-month-old individuals

Table 1 Expression levels of CYP1A1 mRNA in all studied age-groups with statistical analysis
Table 2 Expression of CYP2B1/2 mRNA in all studied age-groups with statistical analysis
Table 3 Expression of CYP3A1 mRNA in all studied age-groups with statistical analysis
Table 4 Activity of NADPH-cytochrome P450 reductase with statistical analysis
Table 5 Activity of NADH-cytochrome b5 reductase with statistical analysis

The lowest constitutive CYP2B1/2 mRNA expression was observed in small intestine of 2-week-old rats, the highest in 2- and 28-month-old animals. Stable and medial level of CYP2B1/2 mRNA was found in 4- and 20-month-old animals. The increase in CYP2B1/2 mRNA level after phenobarbital administration was significant in all studied groups. Although the amount of CYP2B1/2 mRNA in immature rats was low, the inducibility in this age-group was highest (273% of control) and comparable to observed for 4-month animals (266% of control). Significant inducibility was also detected in oldest, 28-month-old rats (208% of control).

The constitutive expression of CYP3A1 mRNA was relatively low in intestinal mucosae from all studied groups of animals. Differences between age-groups were not statistically significant, except 28-month-old rats, where the significant increase in CYP3A1 mRNA expression in comparison with 20-month-old animals was observed (P < 0.005). Dexamethasone did not affect the level of CYP3A1 mRNA in 2-week-old rats; 2- and 4-month-old animals were characterized by higher inducibility of this isoform, 614 and 406% of control, respectively. The highest increase in the amount of CYP3A1 mRNA after dexamethasone induction was found in small intestine of 20- and 28-month-old rats: 2,233 and 1,800% of control, respectively.

The activities of both studied reductases, NADPH-cytochrome P450 and NADH-cytochrome b5, in rat small intestine apparently showed age-dependent fluctuations, the lowest in 2-week-old and the highest in 28-month-old animals. In intestinal mucosa of 28-month-old rats, the activities of the above enzymes were about 3-fold higher than in 4- and 20-month-old animals. Analogous tendencies were observed in all studied groups after treatment with CYP450 inducers as well as changes in the intestinal activities of studied reductases in induced animals were low. Only 20-month-old rats after ÎČ-naphtoflavone administration and 28-month-old animals after phenobarbital treatment showed abundant increase in NADPH-CYP450 reductase activity in comparison with controls (Figs. 4, 5).

Fig. 4
figure 4

Age-related differences in NADPH-cytochrome P450 reductase activity in rat small intestine. Values are expressed as micromoles/min/mg of protein ± S.D. Significant difference at **P < 0.001 and *P < 0.005 versus control 2-week-old rats, at ‡ P < 0.005 and † P < 0.01 versus control 2-month-old rats, at filled circle P < 0.01 versus control 4-month-old rats, at filled diamond P < 0.01 versus control 20-month-old individuals. The differences in the enzymatic activity between the control and induced animals at the same age were not statistically significant, except for 20- and 28-month-old animals treated with ÎČ-naphtoflavone and phenobarbital, respectively. On account of that and also to maintain the lucidity, the graph shows all the values versus control groups only. Complete statistical analysis is shown in Table 4

Fig. 5
figure 5

Age-related differences in NADH-cytochrome b5 reductase activity in rat small intestine. Values are expressed as micromoles/min/mg of protein ± S.D. Significant difference at **P < 0.001 and *P < 0.05 versus control 2-week-old rats, at ‡ P < 0.01 and † P < 0.05 versus control 2-month-old rats, at filled circle P < 0.01 versus control 4-month-old rats, at filled diamond P < 0.01 versus control 20-month-old rats. The differences in the enzymatic activity between the control and induced animals at the same age were not statistically significant, except for 20- and 28-month-old animals treated with ÎČ-naphtoflavone and phenobarbital, respectively. On account of that and also to maintain the lucidity, the graph shows all the values versus control groups only. Complete statistical analysis is shown in Table 5

Discussion

Intestinal biotransformation of drugs and dietary xenobiotics may be modified during maturation and aging. The main purpose of this study was to estimate the level of expression and inducibility of selected intestinal CYP450 mRNAs in various phases of rat life. Biochemical analysis of the cytochrome P450 and cytochrome b5 reductases activity in function with age was the second but also important aim of the presented work. However, it should be explicitly stressed that the results of this experiment do not concern the age-related drug metabolism and disposition in humans. Under conditions of our experiment, constitutive CYP1A1 mRNA expression was lowest in the small intestine of 2-week-old rats and was increased in sexually mature 2-month-old animals. Since the attainment of maturity, the animals showed relatively constant levels of constitutive CYP1A1 mRNA. Such a stable expression persisted till the advanced animal age, when its significant augmentation was observed. These data may indicate that the constitutive intestinal expression of CYP1A1 gene changes during maturation and aging. Inducibility of CYP1A1 gene was evident in 2-, 4- and 20-month-old rats. It is known that the CYP1 family is involved in metabolizing aromatic hydrocarbons to potentially harmful and genotoxic products, the CYP1B1 gene is often overexpressed in colon adenocarcinoma cells (Gibson et al. 2003). The food-derived heterocyclic aromatic amines act as the inducers of intestinal CYP1A1 whereas some components found in Saint John’s wort (Hypericum perforatum), e.g., myricetin, apigenin and quercetin can selectively inhibit this isoform (HĂŒmmerich et al. 2004; Chaudhary and Willett 2006). Relatively high expression and inducibility of intestinal CYP1A1 in aged rats may suggest the existence of analogous pattern in older humans. Perhaps, the flavonoids mentioned above may be considered suitable for administration as chemoprotective and cancer-preventive substances also in aged patients.

Changes in CYP2B1/2 mRNA expression were similar to those observed for CYP1A1, a constitutive mRNA level of this isoform was lowest in 2-week-old rats and highest in 2- and 28-month-old animals. It may reflect the basic activity of CYP2B1/2 in either immature or aged rats; our previous study on the age-related changes in expression of selected intestinal CYP450 proteins showed a parallel profile of the constitutive CYP2B1/2 levels (PaƂasz et al. 2003, also unpublished data). The amount of CYP2B1/2 mRNA increased significantly after phenobarbital administration in all studied age-groups, especially in oldest 28-month-old individuals. These findings compare well with our earlier data showing that the oldest rats exposed had a relatively high inducibility of CYP2B1/2 protein (PaƂasz et al. 2003). Studies performed by Patel et al. (1998) on rat fetuses, newborns and animals in the early period of postnatal life showed significant increases in CYP2B protein levels in the small intestine during sexual maturation. The results of the present study support this observation and also may suggest that the constitutive intestinal expression of CYP2B in sexually immature rats is only slightly marked in comparison with adult ones. It is possible that the CYP2B level in the digestive tract may be modulated by alterations in steroid hormone concentrations, e.g., testosterone (Fujita et al. 1990), although there are still no available investigations confirming this mechanism.

The CYP3A1 isoform, which has particularly high concentration in the rat liver, was confirmed to be also expressed in the small intestine. The mRNA of this isoform exhibited a completely different profile of intestinal expression and inducibility than previously described CYPs. Dexamethasone had no effect on the level of CYP3A1 mRNA in 2-week-old rats. It supports the conjecture that CYP3A1-dependent I phase xenobiotic biotransformation in the small intestine of sexually immature rats may be considerably limited.

These findings were consistent with a previous study in which Warrington et al. (2004) noted no statistically significant age-dependent changes of CYP3A expression in the rat small intestine. A comparable stability was also observed by Wauthier et al. (2004) in constitutive hepatic CYP3A mRNA content in 3-, 8-, 11- and 18-month-old rats. It seems that such isoforms should be less affected by age-related oxidative injuries, e.g., decrease in reduced glutathione concentration. However, interestingly the oldest 28-month-old animals showed a significant increase in intestinal CYP3A1 mRNA expression after dexamethasone administration.

Results published by Lee and Werlin (1995) showed that in the liver of 5-day-old rats treated with dexamethasone, very high CYP3A1 mRNA expression was observed in comparison with adult animals. These data do not correlate with our results concerning rat small intestine, where the CYP3A1 inducibility was highest in oldest, 28-month-old individuals. The differences between small intestine and liver in age-dependent CYP3A protein expression were also reported by other authors (Warrington et al. 2004) who showed that in the liver of aged rats, a significant decrease in CYP3A occurred, whereas the intestinal expression of this isoform was unchanged. George et al. (1995) observed that the level of hepatic CYP3A protein in human decreases during aging. However, our previous results derived from the first experiment clearly showed that the amount of intestinal CYP3A1 protein as well as its inducibility did not decrease even at advanced stage of rat life (PaƂasz et al. 2003). Therefore, it may suggest that the pattern of age-dependent changes in intestinal CYP3A expression is substantially different than observed in the liver. Okabe et al. (2003) studying CYP3A activity in rats after nephrectomy and glycerol or cisplatin intoxication also found that the intestinal expression of this isoform did not change, whereas it significantly decreased in the liver. Assuming that the profile of cytochrome P450-dependent biochemical processes performed by rat intestinal mucosa seems not to be analogous to xenobiotic biotransformation by hepatocytes. Not many food products such as the well-described grapefruit juice act as blockers of this isoform either in rodents or in humans. It seems to be important, that the plasma concentrations of some drugs may be significantly and sometimes dangerously increased by concomitant treatment with this beverage when the medicines are administered orally (Hanley et al. 2011). The well-known members of the CYP3A family are the only isoforms expressed in clinically meaningful amounts in human enteric mucosa. Probably, the parallel profile of the intestinal CYP3A4 isoform action may also take place in older patients.

Reductases, the unique electron donors for catalytic center of CYP450 protein, are important and inseparable components of oxidative phase in xenobiotic biotransformation. The results of our performed study clearly demonstrate that activities of NADPH-cytochrome P450 and NADH-cytochrome b5 reductase in the rat small intestine change in various phases of life. Constitutive activities of both enzymes were lowest in immature 2-week-old rats, and the inducers influenced their activity in this age-group. Nevertheless, this effect was poorly significant. Activity of NADPH-cytochrome P450 reductase in this age-group was slightly decreased after phenobarbital and ÎČ-naphtoflavone administration. On the other hand, dexamethasone increased NADH-cytochrome b5 activity in the small intestine of 2-week-old rats. During sexual maturation, the increase in the activity of studied reductases was evident. After attainment of sexual maturity, the activity of both reductases was relatively stable till the 20-month-old age, and then the increase was evident again. The aged, 28-month-old rats were characterized by the highest activity of both NADPH-CYP450 and NADH-cytochrome b5 reductases. Nevertheless, Warrington et al. (2004) suggested an age-dependent decline in NADPH-CYP450 reductase protein expression in the rat small intestine. However, it is proper to notice that this western blotting and immunohistochemical study did not concern the enzymatic activity of both reductases in the gut microsomal fraction. It was performed on young mature (2 months old) rats only and did not include either immature or extremely aged 28-month-old animals. The age-dependent changes of reductase activity in the rat small intestine are similar to those observed by some authors in the liver (Plewka and Kaminski 1992). Studies dealing with effects of age and phenobarbital on hepatic mixed function monooxygenases showed higher NADPH-CYP450 reductase activity in 2-month-old rats in comparison with 2-week-old and 28-month-old animals. We suggest that in the intestinal mucosa of aged rats as well as other mammals, not excluding humans, the augmentation of NADPH/NADH-dependent oxidoreductive processes take place. These reactions are often connected with the generation of free radicals, leading to injury of various cellular structures, e.g., phospholipid bilayers and nuclear chromatin. It may contribute to dysplastic or even neoplastic transformation of gut mucosa frequently observed in aged mammals. A lot of carcinogenic metabolites are the products of CYP450-dependent biotransformation of various agents, for example, polycyclic hydrocarbons (PAHs) and numerous organic food contaminants, heterocyclic aromatic amines, polyphenols, dioxins, urethane, etc. (HĂŒmmerich et al. 2004; Stupans et al. 2001; Guengerich et al. 1994). High inducibility of CYP1A1, CYP2B1/2 and CYP3A1 genes in the small intestine of aged rats could also promote carcinogenesis within intestinal epithelium. Probably, the CYP1A1 isoform plays a particular role in this process. There are suggestions that biotransformation of PAHs and also food-derived xenobiotics into active carcinogens depends on CYP1A1 gene variability (Shimada and Fujii-Kuriyama 2004). It is generally accepted that the high level of oxidative reactions is an important factor in the course of aging processes. Our results suggest that the phenomenon of intestinal aging is reflected by qualitative and quantitative changes in the expression of particular cytochrome P450 isoforms as well as activities of their reductases. Interestingly, the age of animals influences the expression of CYP1A1, CYP2B1/2 and CYP3A1 in a selective manner. The constitutive level and inducibility of studied cytochrome P450 isoforms in the small intestine of immature rats were very low. Sexually mature animals showed high level expression of CYP450, which was not decreased even at advanced phases of life. Therefore, the expression of CYP450 isoforms in the rat small intestine may be one of the new potential markers of sexual maturity. Some studies on cell proliferation and apoptosis in rat intestinal mucosa showed that the equilibrium of these processes is not significantly impaired during aging (Mandir et al. 2005). It is probably one of the reasons for relatively high metabolic activity in this organ even in old individuals. Other results could also indicate that the intestinal activities of both NADPH-cytochrome P450 reductase and NADH-cytochrome b5 reductase in old rats are higher than in young, mature individuals. We hypothesized that the differences in intestinal biotransforming potential of immature and aged rats may affect the character and rate of dietary xenobiotic metabolism in the gastrointestinal tract. The intestinal metabolic rate as well as the efficiency of cytochrome P450-dependent biotransformation is not decreased by the aging processes. It should be taken into consideration that the high level of oxidative reactions within enterocytes may contribute to pathological changes within the intestinal mucosa of aged animals. Perhaps, these biochemical and cytophysiological processes may be supported or blocked by the presence of various potentially harmful food xenobiotics. This brings up the question of what molecular events regulate activation and inhibition of the selected CYP450 genes involved in intestinal carcinogenesis. We finally postulate that the putative contribution of dietary xenobiotics to this phenomenon requires further study.

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PaƂasz, A., Wiaderkiewicz, A., Wiaderkiewicz, R. et al. Age-related changes in the mRNA levels of CYP1A1, CYP2B1/2 and CYP3A1 isoforms in rat small intestine. Genes Nutr 7, 197–207 (2012). https://doi.org/10.1007/s12263-011-0240-z

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