Abstract

Drug metabolism can be affected by chronic renal failure (CRF). Although it is known that several drugs that are known to be acetylated accumulate in CRF, the effect of CRF on N-acetyltransferase (NAT), the enzyme responsible for this acetylation, is unknown. Herein is reported that protein and gene expression of both Nat isoforms in the liver was reduced by >30% and Nat2 activity was reduced by 50% in rats with CRF compared with control rats. Incubation of hepatocytes with serum from rats with CRF suggested that a circulating factor is responsible for the decrease in protein and gene expression. For testing the hypothesis that parathyroid hormone may be this factor, CRF was induced in parathyroidectomized rats; downregulation of Nat expression and activity was not observed in these rats. Furthermore, addition of parathyroid hormone to cultured hepatocytes induced a decrease in Nat2 protein and gene expression. In conclusion, liver acetylation of drugs in a rat model of CRF is reduced by a downregulation of Nat1 and Nat2 isoforms, secondary to decreased gene expression. Parathyroid hormone seems to be an important mediator of this phenomenon. Reduction in renal function alters the disposition of many drugs mainly by decreasing the elimination of those excreted by the kidney1,2; however, drug metabolism by the liver may also be altered in patients with chronic renal failure (CRF).3 Indeed, several studies have shown that the metabolic clearance of various substrates is reduced in patients with CRF.1–10 Liver enzymes implicated in drug metabolism are classified in phase I (mainly oxidative reaction mediated by cytochrome P450) and phase II (conjugation reactions). Up to now, the studies on the repercussions of CRF on drug metabolism have been primarily focused on cytochrome P450. Indeed, several studies have demonstrated that CRF in rats was associated with a reduction in protein and gene expression as well as a significant decrease in the activity of several liver cytochrome P450 isoforms.11–16 Moreover, we recently reported that this decrease was secondary to uremic circulating factors, particularly parathyroid hormone (PTH).17 Phase II enzymes are also critical for the metabolism of drugs.18,19 These enzymes are responsible for the conjugation of drugs, and glucuronidation mediated by uridine diphosphate-glucuronosyl transferase (UGT) and acetylation mediated by N-acetyltransferases (NAT) are among the most important reactions.19 Interestingly, several human studies have reported a reduction in the liver metabolism of drugs that are cleared by glucuronidation or acetylation in patients with CRF, suggesting that CRF could impede these metabolic pathways.6–9 For instance, zidovudine and morphine (two glucuronidated molecules) have a significantly reduced metabolic clearance in CRF.20,21 Moreover, several drugs extensively acetylated (e.g., isoniazid, procainamide) also accumulate in patients with decreased renal function,2,22–24 suggesting a reduction in hepatic acetylation. Recently, Yu et al.25 showed that liver UGT was unchanged in a CRF rat model; however, no study has been done on the effect of CRF on hepatic acetylation in rat. Human NAT are composed of two isoforms (NAT1 and NAT2), and both are involved in drug metabolism processes, although human NAT1 is also thought to have an endogenous role.26 These enzymes are expressed in the liver; they catalyze acetyl group transfer from acetyl-CoA to an aromatic or heterocyclic amine, hydrazine, hydrazide, or N-hydroxylamine acceptor substrate. NAT metabolize several drugs, such as sulfonamides and isoniazid.26 In the rat, similar to human, there are two isoforms (Nat1 and Nat2), although a third isoform (Nat3) with less metabolic activity was recently characterized.27 The objectives of this study were to determine the effects of CRF on hepatic NAT and to define the mechanisms leading to their downregulation. For this purpose, we measured in control and CRF rats (1) liver Nat1 and 2 protein and gene expression and (2) specific metabolic activity of Nat2. We also evaluated the effects of uremic serum on Nat1 and Nat2 expression by incubating normal rat hepatocytes with control or CRF sera. Finally, the implication of PTH (as a potential uremic factor) in the downregulation of rat Nat genes was also evaluated in vivo in parathyroidectomized rats and in vitro in rat hepatocytes incubated with PTH. RESULTS Biochemical Parameters and Body Weight in Control and CRF Rats Table 1 presents the body weight and the biochemical parameters of the animals studied. As shown, body weights were similar in all groups. CRF rats had higher levels of plasma creatinine and a lower creatinine clearance reduced by 79% (P < 0.001) compared with control rats. Nat Isoforms in the Liver The levels of Nat1 and Nat2 in CRF rat (n = 10) liver were reduced by 33 and 50%, respectively, compared with control animals (P < 0.001; Figure 1). There was a significant negative correlation of Nat protein levels and creatinine clearance (r = 0.76, P < 0.001). To evaluate whether the downregulation of Nat in the liver of CRF rat was secondary to a decrease in the proteins synthesis, we evaluated mRNA encoding the different isoforms by multiplex quantitative PCR. This reveals a significant decrease in mRNA encoding Nat1 and Nat2 in CRF animals (n = 19) compared with controls (n = 16; Figure 2). Thus, the decrease in protein levels of the different Nat isoforms observed in CRF is secondary to reduced gene expression. In Vitro Metabolism of p-Aminobenzoic Acid To determine the repercussion of CRF on the metabolism of drugs by Nat, we assessed the in vitro N-acetylation of p-aminobenzoic acid (PABA; Sigma-Aldrich, Oakville, ON, Canada) in liver cytosols. This enzymatic reaction was mediated primarily by the rat Nat2 isoform. The N-acetylation of PABA was decreased by 50% in rats with CRF (n = 8), compared with control animals (P < 0.001; n = 6; Figure 3). Effects of Uremic Serum on Nat Protein and mRNA Levels The objective of this experiment was to determine the effects of CRF serum on liver Nat. After 48 h of incubation of normal hepatocytes with serum (10%) from rats with CRF (n = 15), the amounts of Nat1 and 2 proteins were decreased by 40 and 57% (P < 0.005), respectively, compared with hepatocytes incubated with serum from control animals (n = 12; Figure 4A). The mRNA levels of Nat1 and Nat2 were both decreased by 30% (P < 0.005; Figure 4B). Thus, uremic serum contains mediators that downregulate Nat expression in normal hepatocytes. Physical and Biochemical Characteristics of Rats with Parathyroidectomy For clarification of the role of PTH in the downregulation of Nat genes, some CRF (n = 6) and control (n = 6) rats were surgically treated to remove parathyroid glands. Table 2 presents the body weight and the biochemical characteristics of the animals used in this experiment. Once again, no difference was observed between groups for body weights, whereas clearance and creatinine were significantly reduced in both CRF groups. There was a 40-fold increase in PTH in CRF rats, confirming the severity of secondary hyperparathyroidism in these animals. PTH was undetectable in rats with parathyroidectomy (PTX). Role of PTH in the In Vivo Downregulation of Rat Nat1 and Nat2 Induced by CRF To determine whether PTH was implicated in the in vivo decrease of Nat by CRF, we evaluated the effects of PTX in CRF rats on Nat1 and 2 protein levels. As shown in Figure 5, preventing the development of secondary hyperparathyroidism by PTX prevents the negative effect of CRF on Nat2 protein and the Nat2 gene. We also observed a significant difference in Nat2 metabolic activity in CRF rats with PTX compared with CRF rats (Figure 5). Similar results were obtained for Nat1 (Figure 6). In Vitro Effect of PTH on Nat2 in Cultured Hepatocytes To confirm the implication of PTH in the downregulation of Nat2 in CRF, we incubated normal hepatocytes during 48 h with 10−9 M synthetic 1-34 rat PTH (n = 12). As shown on Table 2, this concentration of PTH is similar to the one observed in vivo in our CRF rats. The effects of PTH on the Nat2 protein and mRNA levels are shown on Figure 7. When hepatocytes where incubated with PTH, Nat2 protein and Nat2 mRNA levels were decreased by 80% (P < 0.01) and 25% (P < 0.01), respectively. There was no effect of PTH on other control hepatocyte proteins (glyceraldehyde 3-phosphate dehydrogenase, aspartate aminotransferase, or β-actin; data not shown). Although PTH could act via several signaling pathways, we tested the hypothesis that the downregulation of Nat2 was through activation of NF-κB, as previously shown for CYP450.17 Addition of 30 μM andrographolide to hepatocytes cultured in the presence of 10−9 M PTH (n = 6) prevented the decrease in Nat2 gene expression induced by PTH with a subsequent effect on Nat2 protein level (Figure 7). DISCUSSION This study demonstrates that in the rat, CRF induces a marked decrease in liver protein levels of Nat1 and Nat2 isoforms, secondary to a reduction in the levels of mRNA encoding these proteins. The repercussions on the metabolism of drugs by the liver are important, because we observed a 50% reduction of PABA metabolism mediated by Nat2 isoform. The mechanism underlying the downregulation of Nat genes is the presence of endogenous inhibitors in the uremic blood, PTH being one of the major inhibitors. Enzymatic reactions leading to drug biotransformation are classified in phase I and phase II reactions. Phase I reactions usually convert parent drugs to a more polar metabolite and are mediated by cytochrome P450. Parent drugs or their phase I metabolites could also undergo conjugation reactions with an endogenous substrate, such as glucuronic acid, acetic acid, or sulfuric acid, to yield drug conjugates. The two major phase II reactions implicated in drug metabolism are glucuronidation, mediated by UGT, and acetylation, mediated by Nat. Renal failure has been generally thought mainly to decrease the renal clearance of drugs1,2; however, many studies have demonstrated that humans with CRF also present decreased hepatic drug metabolism.1–10 Because the cytochrome P450 is the major enzymatic system involved in drug biotransformation, most studies have focused on liver P450. The results of these studies showed that in CRF rats, liver total P450, several P450 isoforms,11–16,28 and enzymatic reactions normally carried by the liver P450 are significantly decreased.10 We also showed that both patients’ and rats’ uremic serum contain mediators that downregulate liver P450.29,30 Many drugs commonly used in clinical practice are metabolized by phase II enzymes. Several pharmacokinetics studies have revealed a decrease in glucuronidation or acetylation of drugs in patients with CRF, suggesting that not only P450 could be altered in CRF but also phase II enzymes. For instance, the metabolism of zidovudine and metoclopramide, which is primarily mediated by glucuronidation, is reduced in patients with renal failure.20,31,32 Acetylation also seems to be reduced in patients with CRF; several reports have demonstrated that the metabolic clearance of procainamide is reduced by approximately 60% in renal failure.2,23,24 Moreover, a decrease in the acetylation of isoniazid has been reported in patients with CRF.22 The mechanism leading to a decrease in phase II enzymatic reactions in CRF is unknown. Although many animal studies have been done on P450, very few have been performed on the effects of CRF on phase II enzymes. Paterson and Cohn14 studied the uridine diphosphate (UDP)-glucuronyl transferase activity in microsomes from control rats and rats with CRF and reported a 19% reduction in UDP-glucuronyl transferase activity, although this difference was NS (P = 0.06). More recently, Yu et al.25 did not confirm these results: They found no significant difference in liver UGT in CRF rats compared with control rats, although the number of animals was small (n = 4 per group) and the degree of renal failure was moderate. Taburet et al.,33 however, reported that incubation of microsomes, prepared from healthy human livers, with serum of patients with CRF was associated with a decrease in the metabolism of zidovudine, reflecting an inhibition of UDP-glucuronosyltransferase and suggesting that uremic mediators are responsible for the reduction in drug metabolism. Our study is the first to evaluate the effects of CRF on acetylation of drugs. Our results demonstrate a significant decrease in both Nat1 and Nat2 with a major impact on their in vitro activity. Interestingly, we found a strong correlation between creatinine clearance and protein expression, suggesting that as renal function decreases, downregulation of Nat is more important. As shown for CYP450, the mechanism of protein downregulation is secondary to a reduced gene expression. These results could explain why the clearance of drugs cleared by acetylation is reduced in patients with CRF. Another hypothesis to explain decreased drug metabolism in CRF have been raised by Sun et al.,34,35 who demonstrated that hepatic uptake of erythromycin (a CYP450 substrate) by hepatocytes incubated with uremic toxins was decreased. Because uptake by hepatic transporters (e.g., organic anion transporter protein) is the first step in the elimination of several drugs, making it available for metabolizing enzymes, a decrease in organic anion transporter protein as shown in hepatocytes incubated with uremic toxins and more recently in CRF rats could probably explain in part the decrease in drug metabolism induced by CRF.34–36 In this study, we found a decrease in Nat activity using cytosolic preparations that only reflect the metabolic activity and not the uptake or the efflux of drugs that could also be modulated in CRF. In this study, we tested the hypothesis that uremic mediators were implicated in the decrease of NAT in CRF. The results clearly demonstrate that uremic serum contains mediators that are able to downregulate hepatic NAT. Interestingly, the results obtained with uremic serum also closely mimic what we showed in vivo in rats with CRF (Figures 1 and 4). Our results also demonstrate that there is an association between lower levels of Nat mRNA and the corresponding protein (Figure 4) in hepatocytes incubated with serum from rats with CRF. This suggests that gene expression is reduced by mediators present in uremic serum. Although the mechanisms responsible for the diminished hepatic gene expression in CRF are not known, this study suggests that uremic mediator(s) could affect NAT promoters. CRF is often associated with secondary hyperparathyroidism. High levels of PTH have been linked to impaired protein synthesis, by reduced gene expression, in the liver, the skeletal muscle, and the cardiomyocytes.37–39 More recently, we also showed that PTH was an important factor implicated in the decreased of liver P450 in CRF.17 In this study, we tested the hypothesis that PTH could also be implicated in the decrease in liver acetylation. First, we evaluated whether PTX could prevent the downregulation of Nat genes. As shown in Figures 5 and 6, CRF rats with PTX have essentially the same level and metabolic activity of Nat as control rats, demonstrating that PTH is a major in vivo mediator of CRF-induced downregulation of Nat2. Moreover, our results demonstrate that PTH could decrease Nat2 gene expression and cause a corresponding reduction in Nat2 protein in normal hepatocytes (Figure 7). Our results emphasize the deleterious effects of PTH on protein synthesis by the liver. The signaling pathway through which this occur remains poorly described. PTH could act by an increase in cAMP or intracellular calcium.40,41 More recently, we suggested that PTH could also act by activation of NF-κB to downregulate liver CYP450.17 In this study, we also demonstrated that inhibiting the activation of NF-κB prevents the decrease of Nat activity induced by PTH in culture hepatocytes. Further studies are needed to elucidate the effect of PTH on NAT and to investigate further the possible role of transcription factors including NF-κB. In conclusion, this study demonstrated that CRF induces a decrease in rat Nat1 and Nat2 protein secondary to a decrease in gene expression. We also found a major reduction of Nat2 activity, which could explain the decrease in drug acetylation observed in patients with CRF. As shown for other major liver enzymes, the results of this study emphasize that uremic serum contains mediators that downregulate hepatic protein synthesis. PTH seems to be a major culprit in hepatocellular dysfunction in CRF. CONCISE METHODS Experimental Model Male Sprague-Dawley rats (Charles River, Saint-Charles, PQ, Canada) that weighed 200 to 300 g were housed in the Research Center animal care facility and maintained on Harlan Teklad rodent diet (Harlan Teklad Global Diets, Montreal, PQ, Canada) and water ad libitum. All of the experiments were conducted according to the Canadian Council on Animal Care guidelines for care and use of laboratory animals and under the supervision of our local animal care committee. CRF was induced by two-stage five-sixths nephrectomy as previously reported.15 Control rats were pair-fed the same quantity of rat chow that was ingested by the rats with CRF on the previous day. At day 41 after the nephrectomy, the rats were housed in metabolic cages and urine was collected for 24 h to determine the clearance of creatinine. Rats were killed by decapitation at 42 d after nephrectomy. Blood and tissues were stored at −80°C up to analysis. Total PTX was performed, as described previously,17,37 7 d before the first nephrectomy. For avoidance of hypocalcemia, rats were then supplemented in calcium by addition of calcium gluconate to drinking water (control 2.5%; CRF 5%). Control rats received sham surgery in the neck region. Primary Hepatocyte Culture Hepatocytes were isolated from normal rats according to the modified two-step liver perfusion method of Seglen as previously published.29 Collagenase type 4 (Worthington, Lakewood, NJ) was used. Isolated hepatocytes were plated and cultured in 2 ml of William E medium containing 10% of serum from rats with CRF or from control animals. The serum of one rat was used for one experiment. Hepatocytes were incubated during 48 h and were then harvested by scraping. Samples were stored at −80°C up to analysis. To assess whether liver Nat2 could be downregulated by PTH, we measured the ability of rat synthetic 1-34 PTH (Sigma-Aldrich) to depress the Nat of normal hepatocytes. The concentration of PTH used was 10−9 M. Incubation time was 48 h (medium was changed completely after 24 h to maintain PTH concentration). To determine whether NF-κB pathway could be involved in the effect of PTH on Nat2, we blocked this pathway using andrographolide (Calbiochem, San Diego, CA), a widely known NF-κB inhibitor.42 Liver Cytosol Preparation Cytosols were prepared according to the method of Schneck et al.43 with slight modifications. Western Blot Analysis Nat1 and Nat2 were assessed by Western blotting according to a previously published procedure.44,45 Rat Nat2 was detected using a specific polyclonal rabbit antiserum, raised against the C-terminal dodecapeptide common to human NAT1 and mouse and rat Nat2 as described previously.46 β-Actin was detected using a mouse anti-chicken β-actin (Neo-Markers, Fremont, CA). Immune complexes were revealed by peroxidase-conjugated AffiniPure Goat Anti-Rabbit IgG (Jackson ImmunoResearch Laboratories, West Grove, PA) and goat anti-mouse IgG coupled to peroxidase (Sigma-Aldrich), respectively. Rat Nat1 was detected using rabbit anti-rat antibodies recognizing both Nat1 and 2. For achievement of a specific quantification of rat Nat1, the Nat2 isoform is immunoprecipitated before SDS-gel electrophoresis. Cytosols were diluted 1:1 with IP buffer pH 7.4 (300 mM NaCl, 20 mM Tris, 2 mM EDTA, 2 mM EGTA and to which was were incubated with the same of Protein PQ, Canada) for at and then for 1 to the The was incubated with for 2 h at Protein was to the and incubation was at were by and were up to of rat Nat1 by Western and Analysis Total were from liver and hepatocytes by using the and ON, respectively. and for rat Nat1 and and for were used for quantitative analysis. data were by the of Nat2 The metabolic activity of rat Nat2 in treated hepatocytes or cytosolic liver of the different groups of rats was on the of the method described by et which has been modified by and The method the of are incubated with and were in of Rat PTH PTH was measured by using the Rat PTH which the PTH. The level is Analysis The results are expressed as between groups were assessed by using or an by The of was P < Protein expression of liver Nat1 and 2 in control and CRF rats. Control results were as are are shown in < of liver Nat1 and 2 mRNA in and CRF rats. Control results were as are < Nat2 metabolizing activity as measured by using PABA as specific in and CRF rats liver. expressed by of per of protein per are < and Protein and mRNA expression of Nat1 and Nat2 in cultured hepatocytes incubated with and CRF rat serum in hepatocytes incubated with serum was as are shown in are P < rats; < of Nat2 protein mRNA and activity in and CRF rat liver with or rats were as are are shown in P < control rats; P < CRF of Nat1 protein and mRNA in and CRF rat liver with or rats were as are are shown in P < Protein and mRNA expression of Nat2 in hepatocytes incubated for 48 h with 10−9 M PTH in 10% serum with or 30 μM andrographolide of incubated with serum PTH and andrographolide were as are are shown in P < P < PTH characteristics of characteristics of rats with was by the Canadian of Research and is a of the the for of this was at the of the for the of to