α-Lipoic acid is a natural compound that is widely distributed in plants and animals and functions as a cofactor within mitochondrial enzymes to catalyse the oxidative decarboxylation of α-keto acids (such as pyruvate dehydrogenase and α-ketoglutarate dehydrogenase) and the cleavage of glycine( Reference Shay, Moreau and Smith 1 , Reference Wollin and Jones 2 ). Besides its role in the mitochondrial metabolic pathway, α-lipoic acid, when supplemented in diets, performs various physiological activities in experimental animals( Reference Shay, Moreau and Smith 1 , Reference Wollin and Jones 2 ) and is widely used as a dietary supplement by humans. However, the concentration of α-lipoic acid in natural food items is very low( Reference Durrani, Schwartz and Nagl 3 ). Therefore, dietary α-lipoic acid supplements are manufactured by chemical synthesis. It has been well established that dietary α-lipoic acid is effective at attenuating oxidative stress( Reference Shay, Moreau and Smith 1 , Reference Wollin and Jones 2 , Reference Amudha, Josephine and Varalakshmi 4 – Reference Xu, Gao and Song 8 ). Many studies have also indicated that α-lipoic acid modulates glucose metabolism and is effective at ameliorating insulin resistance and attenuating type 2 diabetes( Reference Shay, Moreau and Smith 1 , Reference Bilska and Włodek 6 , Reference Henriksen, Diamond-Stanic and Marchionne 7 ). The lipid-lowering property of α-lipoic acid has also frequently been reported( Reference Wollin and Jones 2 , Reference Yi and Maeda 9 – Reference Ford, Cotter and Cameron 11 ). In this context, we had previously demonstrated that α-lipoic acid strongly reduces the activity and mRNA levels of hepatic lipogenic enzymes in rats( Reference Huong and Ide 12 – Reference Ide, Azechi and Kitade 14 ). Therefore, the reduction in hepatic lipid biosynthesis may account for the lipid-lowering effect of α-lipoic acid. During the course of the studies, we had found that dietary α-lipoic acid lowers serum concentrations of TAG, cholesterol and phospholipids and hepatic concentrations of TAG and cholesterol, but increases the hepatic concentration of phospholipids. The increased hepatic concentration of phospholipids implies that α-lipoic acid causes biomembrane proliferation in this tissue. We hypothesise that α-lipoic acid is an inducer of hepatic drug-metabolising enzymes because drugs that induce hepatic drug metabolism also increase phospholipid concentration and synthesis in this tissue accompanying the proliferation of the endoplasmic reticulum( Reference Orrenius and Ericsson 15 ). In relation to this, some studies( Reference Jia, Hallur and Zhu 16 – Reference Ki and Kim 18 ) have shown that α-lipoic acid increases the mRNA expression or activity or the protein concentrations of drug-metabolising enzymes in cultured cells. However, information on the effect of α-lipoic acid on drug-metabolising enzymes in experimental animals is lacking. In this context, we investigated the effect of dietary α-lipoic acid on the gene expression of hepatic enzymes involved in drug metabolism in rats in the present study, employing DNA microarray analysis, a powerful technique for analysing the mRNA expression of thousands of genes in a short period of time. Drug metabolism usually involves many isoenzymes differing in substrate specificity. A considerable number of isoenzymes are relatively irrelevant and only a small number are sensitive to dietary factors( Reference Odbayar, Kimura and Tsushida 19 ). Therefore, microarray-based profiling of gene expression helps to clarify the overall picture of the physiological effect of α-lipoic acid on the mRNA expression of enzymes involved in drug metabolism and to identify isoenzyme(s) specifically affected by this compound.
Materials and methods
Animals and diets
Male Sprague–Dawley rats obtained from Charles River Japan at 4 weeks of age were housed individually in animal cages in a room with controlled temperature (20–22°C), humidity (55–65 %) and lighting (lights on from 07.00 to 19.00 hours) and fed a commercial non-purified diet (Type NMF; Oriental Yeast Company) for 7 d. After this acclimatisation period, the rats were randomly divided into four groups with equal mean body weights, consisting of seven animals each, and fed purified experimental diets containing 0, 0·1, 0·25 and 0·5 % (w/w) of R/S-α-lipoic acid for 21 d. Rats are widely used as an animal model for humans to evaluate the physiological activity of dietary factors. The basal composition of the experimental diets was as follows (in wt%): palm oil, 10; casein, 20; maize starch, 15; cellulose, 2; mineral mixture (AIN-93G-MX)( Reference Reeves, Nielsen and Fahey 20 ), 3·5; vitamin mixture (AIN-93-VX)( Reference Reeves, Nielsen and Fahey 20 ), 1·0; l-cystine, 0·3; choline bitartrate, 0·25; sucrose, 100 g. There were 15 g of dl-α-tocopherol acetate in 1 kg of AIN-93-VX. HPLC analysis revealed that 1 kg of palm oil contained 0·164 g of d-α-tocopherol and 0·0059 g of d-γ-tocopherol. Therefore, all the experimental diets contained 0·015 % (w/w) dl-α-tocopherol acetate, 0·016 % (w/w) d-α-tocopherol and 0·0006 % (w/w) d-γ-tocopherol as antioxidants. Although the AIN-93G diet formula recommended by the American Institute of Nutrition( Reference Reeves, Nielsen and Fahey 20 ) is suggested to provide 0·0014 % (w/w) tert-butylhydroquinone as an antioxidant, we did not use this compound in the present study. Chemically synthesised R/S-α-lipoic acid with purity exceeding 990 g/kg (manufacturer's statement) was purchased from Tokyo Chemical Industry. Enantioselective HPLC analysis( Reference Niebch, Büchele and Blome 21 ) using 11-mercaptoundecanoic acid as an internal standard revealed that the R/S-α-lipoic acid preparation contained 45·9 and 54·1 % (w/w) of R-isomers and S-isomers, respectively. Varying amounts of α-lipoic acid were added to the diets at the expense of sucrose. This resulted in a decrease in the energy content of the experimental diets. However, this decrease was very small (less than 0·23 % of the total energy of the diets). Upon completion of the experimental period, the rats were anaesthetised using diethyl ether and killed by bleeding from the abdominal aorta, after which the livers were excised. The present study was approved by the review board of animal ethics of our institute, and we followed the institute's guidelines in the care and use of laboratory animals. We read and followed the ARRIVE (Animal Research: Reporting In Vivo Experiments) guidelines for animal research (http://www.nc3rs.org.uk/page.asp?id = 1357) in conducting the animal experiment and in preparing the manuscript.
Affymetrix GeneChip and GeneSpring analyses
Hepatic RNA was extracted according to the method of Chomczynski & Sacchi( Reference Chomczynski and Sacchi 22 ). RNA from the livers of six rats fed diets containing 0 and 0·5 % (w/w) α-lipoic acid each was subjected to microarray analyses. Rats with the lowest body weights in each group at the time of killing were excluded from the microarray analyses. RNA was processed using kits supplied by Affymetrix to prepare fragmented biotinylated complementary RNA for hybridisation to the Rat Genome 230 2.0 Array. DNA microarray data were analysed using the GeneSpring GX version 7.3 software (Agilent Technologies, Inc.). Normalisations per chip and per gene were carried out using the 50th percentile value of signal intensity in each chip and the mean values in rats fed a control diet free of α-lipoic acid, respectively. After normalisation, the following filtering criteria were adopted to prepare the gene list for subsequent analysis to eliminate unreliable data with low signals: the expression data had to call more than six P- or M-flags according to the Affymetrix algorithm out of twelve measurements and the average signal intensity had to be greater than 100 in each treatment. The expression data of 12 335 genes fulfilled these criteria. Fold changes in the expression of genes in rats fed the diet containing 0·5 % (w/w) α-lipoic acid compared with the values in rats fed the diet free of this compound were evaluated using this gene list.
Real-time PCR quantification of mRNA
The real-time PCR quantification of mRNA was carried out as described previously( Reference Ide 23 ) in rats fed diets containing 0, 0·1, 0·25 and 0·5 % (w/w) α-lipoic acid. The abundance of mRNA was calculated as a ratio to the abundance of β-actin mRNA in each complementary DNA sample and expressed as a fold change, assigning a value of 1 for rats fed the diet free of α-lipoic acid. The mRNA levels of the aldehyde dehydrogenase 1 family, member A1 (Aldh1a1), aldo-keto reductase family 1, member D1 (Akr1d1), aldo-keto reductase family 7, member A3 (Akr7a3), cytochrome P450, family 2, subfamily b, polypeptide 12 (Cyp2b12), cytochrome P450, family 4, subfamily b, polypeptide 1 (Cyp4b1), epoxide hydrolase 1, microsomal (Ephx1), flavin-containing monooxygenase 5 (Fmo5), glutamate–cysteine ligase, modifier subunit (Gclm), glutamate–cysteine ligase, catalytic subunit (Gclc), glutathione reductase (Gsr), glutathione S-transferase alpha 3 (Gsta3), glutathione S-transferase pi 1 (Gstp1), glutathione S-transferase theta 1 (Gstt1), glutathione S-transferase theta 3 (Gstt3), metallothionein 1a (Mt1a) and NAD(P)H dehydrogenase, quinone 1 (Nqo1) were measured using the TaqMan probe PCR method as described in the handbook (Real-time PCR Systems Chemistry Guide) supplied by Applied Biosystems. The nucleotide sequences of primers and probes used for detecting these mRNA were designed using the Primer Express Software (Applied Biosystems), and these are listed in Table 1. The mRNA levels of the ATP-binding cassette, subfamily B, member 1A (Abcb1a), ATP-binding cassette, subfamily C, member 4 (Abcc4), carboxylesterase 2C (Ces2c), glutathione peroxidase 2 (Gpx2), nuclear receptor subfamily 1, group I, member 3 (Nr1i3), sulfotransferase family, cytosolic, 1C, member 2 (Sult1c2) and UDP-glucuronosyltransferase 2 family, polypeptide B1 (Ugt2b1) were measured using the SYBR Green PCR method. Forward and reverse primers used for detecting these mRNA were designed, prepared and provided by Takara Bio, Inc. The reaction specificity for this method was verified by a melting curve analysis. The nucleotide sequences of primers are also listed in Table 1.
Enzyme assays
About 2·5 g of each liver sample were homogenised with 15 ml of 0·25 m-sucrose containing 1 mm-EDTA and 3 mm-Tris–HCl (pH 7·2) and centrifuged at 200 000 g for 30 min. The activities of Gst and Gsr were measured spectrophotometrically using 200 000 g supernatant as an enzyme source. The activity of Gst was assayed using 1-chloro-2,4-dinitrobenzene, 1,2-dichloro-4-nitrobenzene, p-nitrobenzyl chloride and ethacrynic acid as substrates. The respective conditions (concentrations of substrates and pH) under which enzyme activity was determined using these substrates were the same as those described by Habig & Jakoby( Reference Habig and Jakoby 24 ). The activity of Gsr was measured according to the method described by Carlberg & Mannervik( Reference Carlberg and Mannervik 25 ).
Analyses of serum and liver components
For the determination of hepatic glutathione concentration, about 1·5 g of liver sample were homogenised with 4·5 ml of 8 % perchloric acid and centrifuged at 15 000 g for 30 min. The supernatants (4 ml each) were neutralised with 3 m-K2CO3. After allowing to stand in ice for 10 min, the mixtures were centrifuged at 3000 g for 10 min. The supernatants were used to determine glutathione concentration by the method of Anderson( Reference Anderson 26 ). Malondialdehyde in the serum and liver samples was analysed by HPLC as thiobarbituric acid adducts( Reference Khoschsorur, Winklhofer-Roob and Rabl 27 ).
Statistical analysis
Microsoft Excel add-in software (Excel Statistics 2010, Social Survey Research Information Company) was used for statistical analysis. The constancy of the variance and normality of the distribution of the observations were evaluated using Levene's test and the Kolmogorov–Smirnov test, respectively. If variances were heterogeneous and/or the distributions were not normal, they were transformed logarithmically. The transformations were successful in rendering the variance of the observation constant and the distribution of data normal, and hence the transformed values were used for subsequent statistical evaluations. Significant differences in the means for microarray data at a level of P< 0·05 were evaluated with two-sided Student's t test. The other data were analysed with one-way ANOVA to establish whether the effect of α-lipoic acid was significant, and significant differences in the means at a level of P< 0·05 were evaluated with two-sided Tukey's test.
Results
Growth parameters and liver weight
α-Lipoic acid at a dietary level of up to 0·25 % (w/w) did not affect food intake (Table 2). However, the diet containing 0·5 % (w/w) α-lipoic acid compared with the diet free of this compound significantly reduced this parameter. Growth was significantly lower in rats fed diets containing 0·25 and 0·5 % (w/w) α-lipoic acid than in those fed the α-lipoic acid-free diet. The diet containing 0·1 % (w/w) α-lipoic acid did not affect this parameter. Liver weights were the same among rats fed diets containing 0, 0·1 and 0·25 % (w/w) α-lipoic acid. However, this parameter was significantly higher in rats fed the diet containing 0·5 % (w/w) α-lipoic acid than in those fed the α-lipoic acid-free diet.
Mean values were significantly different from those of rats fed the α-lipoic acid-free diet: * P< 0·05; ** P< 0·01.
Microarray analysis of mRNA expression
Considerable numbers of genes were affected by dietary α-lipoic acid. In total, 997 and 1074 of the 12 335 filtered genes were found to be up-regulated and down-regulated, respectively, more than 1·5-fold by the diet containing 0·5 % (w/w) α-lipoic acid. The numbers of genes up-regulated and down-regulated more than 2-fold by α-lipoic acid were 410 and 245, respectively. We had previously reported that α-lipoic acid reduces the activity and mRNA levels of many enzymes involved in lipogenesis in the liver( Reference Huong and Ide 12 – Reference Ide, Azechi and Kitade 14 ). Consistent with this observation, in the present study using DNA microarray analysis, we observed that α-lipoic acid down-regulated many genes related to lipogenesis more than 1·5-fold. These included the patatin-like phospholipase domain containing 3 (Pnpla3; four probes detected the mRNA levels of this protein and the values assigning a value of 1 for rats fed the diet free of α-lipoic acid were in the range of 0·052–0·081), fatty acid synthase (Fasn; the values for two probes were 0·125 and 0·251), acetyl-CoA carboxylase-α and -β (Acaca and Acacb; the values for two probes were 0·350 and 0·438 and 0·166 and 0·188, respectively), ELOVL fatty acid elongase-2, -5 and -6 (Elovl2, -5 and -6; 0·337 and 0·505 for Elovl2 and -5, respectively, and 0·213 and 0·250 for Elovl6 for two probes, respectively), pyruvate kinase, liver and red blood cell (Pklr; 0·351), thyroid hormone-responsive protein (Thrsp; 0·383 and 0·506 for two probes), phosphogluconate dehydrogenase (Pgd; 0·403), stearoyl-CoA desaturase 1 (Scd1; 0·458), glycerol-3-phosphate acyltransferase, mitochondrial (Gpam; 0·467 and 0·619 for two probes), glucose-6-phosphate dehydrogenase (G6pd; 0·504), ATP citrate lyase (Acly; 0·519 and 0·532 for two probes), fatty acid desaturase-1 and -2 (Fads1 and -2; 0·566 and 0·541, respectively), malic enzyme 1 (Me1; 0·561 and 0·600 for two probes) and SREBF chaperone (Scap; 0·575).
In addition to the lipogenic pathway, we found that genes involved in drug metabolism and the antioxidation system were targeted by dietary α-lipoic acid. Table 3 lists the genes affected more than 1·5-fold by the diet containing 0·5 % (w/w) α-lipoic acid. The drug metabolism pathway has generally been grouped into phase I reactions, in which enzymes carry out oxidation, reduction or hydrolysis reactions; phase II reactions, in which enzymes form a conjugate of the substrate; and phase III reactions, in which enzymes transport drugs. α-Lipoic acid apparently increased the mRNA expression of many phase I enzymes that catalyse oxidation (Cyp4b1, Cyp2b12 and Fmo5), reduction (Akr7a3, Aldh18a1, Aldh1a7, Akr1c1, Aldh1a1, Akr1d1 and Nqo1) and hydrolysis reactions (Ces2c and Ephx1). This compound also increased mRNA expressions of phase II enzymes that catalyse glutathione conjugation (Gsta3, Gstt3, Gstp1, Gstt1 and Gsto1), sulfation (Sult1c2) and glucuronidation (Ugt2b1 and Ugt1a). The mRNA expression of some phase III transporters, including Abcb1a, ATP-binding cassette, subfamily B, member 1B (Abcb1b), Abcc4 and ATP-binding cassette, subfamily A (ABC1), member 8 (Abca8), was also up-regulated by α-lipoic acid. Nr1i3 is a member of the nuclear receptor superfamily and activates many genes involved in drug metabolism( Reference Tolson and Wang 28 ). α-Lipoic acid increased the mRNA expression of this transcription factor.
Mean values were significantly different from those of rats fed the α-lipoic acid-free diet: * P< 0·05; ** P< 0·01.
We also observed that α-lipoic acid increased the mRNA expression of miscellaneous proteins involved in the antioxidation system. Metallothionein is a cysteine-rich protein that has marked capacity to bind metal ions. This protein controls metal ion homeostasis and prevents the toxicity of heavy metals. Metallothionein has also been found to perform diverse functions. In particular, this protein has been considered to be a key component of cellular defence against oxidative stress( Reference Swindell 29 ). In rats, four types of the metallothionein gene, termed Mt1a, metallothionein 2A (Mt2A), Mt3 and Mt4, have so far been discovered. α-Lipoic acid at a dietary level of 0·5 % (w/w) caused about a 10-fold increase in the mRNA expression of Mt1a and Mt2A. In organisms, two systems are considered critical for general reduction–oxidation (redox) regulation, the thioredoxin and glutaredoxin (Glrx)/glutathione systems( Reference Luo, He and Kelley 30 ). Thioredoxin and thioredoxin reductase and Glrx, glutathione and Gsr represent primary components of the former and latter systems, respectively. In rats, three forms of thioredoxin reductase have been identified (Txnrd1–3). α-Lipoic acid caused more than a 2-fold increase in the mRNA expression of Txnrd1 in the present study. Among the proteins involved in the Glrx/glutathione system, α-lipoic acid increased the mRNA expression of Gsr, Gclc (a heavy catalytic subunit of glutamate–cysteine ligase that catalyses the first step of glutathione synthesis) and the mitochondrial isoform of Glrx (Glrx2), but unexpectedly decreased the mRNA expression of the cytosolic form of Glrx (Glrx1). Although the magnitude of the increase did not exceed 1·5-fold, α-lipoic acid also caused a significant increase in the mRNA expression of a light regulatory subunit of glutamate–cysteine ligase (Gclm) (1·00 (sem 0·056) and 1·45 (sem 0·09) in rats fed the α-lipoic acid-free diet and the diet containing 0·5 % (w/w) α-lipoic acid, respectively). The peroxiredoxins function as cysteine-dependent thiol peroxidases that detoxify H2O2 and lipid peroxides and hence exert cytoprotective and antioxidative effects. Under increased oxidative stress, the cysteine moiety of peroxiredoxins is hyperoxidised to sulfinic acid and hence they lose their peroxidase activity. This inactive form can be reduced back to the active thiol form by sulfiredoxin 1 (Srxn1), an ATP-dependent reductase( Reference Soriano, Baxter and Murray 31 ). The mRNA expression of this reductase was found to be up-regulated by α-lipoic acid in the present study. APEX nuclease 1 (Apex1) is a DNA repair protein that also functions as a redox regulator in mammals( Reference Luo, He and Kelley 30 ). α-Lipoic acid caused a 2·5-fold increase in the mRNA expression of this protein. Glutathione peroxidase catalyses the reduction of hydroperoxides and H2O2 by glutathione and thereby protects against oxidative damage. So far, eight different isoforms of glutathione peroxidase have been identified in humans (GPX1–8) and rodents (Gpx1–8). Microarray analysis indicated that α-lipoic acid increased the mRNA expression of Gpx2 but not of other Gpx isoforms.
Real-time PCR analysis of mRNA expression and determination of enzyme activities
The observations made with DNA microarray analysis revealed that dietary α-lipoic acid increased the mRNA expression of proteins involved in drug metabolism and attenuation of oxidative stress. To confirm this observation, we analysed mRNA expression by real-time PCR analysis in rats fed diets containing varying amounts of α-lipoic acid. The observations made with real-time PCR analysis essentially confirmed those made with DNA microarray analysis. In fact, α-lipoic acid dose dependently increased the mRNA expression of phase I enzymes (Cyp2b12, Cyp4b1, Fmo5, Akr1d1, Akr7a3, Aldh1a1, Nqo1, Ces2c and Ephx1) (Fig. 1), phase II enzymes (Gsta3, Gstp1, Gstt1, Gstt3, Ugt2b1 and Sult1c2) and phase III transporters (Abcb1a and Abcc4) (Fig. 2). We also confirmed that α-lipoic acid even at a dietary level of 0·1 % (w/w) significantly increased the mRNA expression of Nrli3. The magnitudes of the increase observed in rats fed the diet containing 0·5 % (w/w) α-lipoic acid generally approximated those observed with DNA microarray analysis except for a few genes (Ces2c, Gsta3 and Sult1c2). The extent of changes in the expression of these genes induced by α-lipoic acid was considerably lower when the values were obtained using real-time PCR than when obtained using DNA microarray analysis.
As α-lipoic acid increased the mRNA expression of some Gst isoenzymes, we analysed the activity of Gst using four different substrates (1-chloro-2,4-dinitrobenzene, 1,2-dichloro-4-nitrobenzene, p-nitrobenzyl chloride and ethacrynic acid). The enzyme activity measured using 1-chloro-2,4-dinitrobenzene as a substrate was significantly higher in rats fed diets containing various amounts of α-lipoic acid than in those fed the diet free of this compound (Fig. 3). The activity of the enzyme measured using this substrate was about 1·5 times higher in rats fed the diet containing 0·5 % (w/w) α-lipoic acid than in those fed the diet free of this compound. Significant but less prominent increases in enzyme activity were also observed when 1,2-dichloro-4-nitrobenzene was used as a substrate in rats fed diets containing 0·25 and 0·5 % (w/w) α-lipoic acid than in those fed the α-lipoic acid-free diet. However, significant increases in enzyme activity in rats fed diets containing various amounts of α-lipoic were not observed when using p-nitrobenzyl chloride and ethacrynic acid as substrates (data not shown).
In Fig. 4(a), the effect of dietary α-lipoic acid on the mRNA levels of proteins involved in the thiol redox regulation system and Mt1a analysed by real-time PCR analysis among rats fed diets containing varying amounts of α-lipoic acid is shown. The results obtained using DNA microarray analysis were generally confirmed using real-time PCR analysis; that is, dietary α-lipoic acid dose dependently increased the mRNA levels of Gsr, Gpx2, Gclc, Gclm, Glrx2, Txnrd1, Srnx1 and Apex1. The decrease in the mRNA expression of Glrx1 caused by the diet containing 0·5 % (w/w) α-lipoic acid observed using DNA microarray analysis was also observed using real-time PCR analysis. However, the decrease was considerably attenuated when the parameter was analysed using real-time PCR analysis. A significant decrease in this parameter was not confirmed in rats fed diets containing 0·1 and 0·25 % (w/w) α-lipoic acid. As α-lipoic acid increased the mRNA expression of subunits of a rate-limiting enzyme in glutathione biosynthesis, we measured hepatic glutathione concentration (Fig. 4(b)). Dietary α-lipoic acid dose dependently increased this parameter, and values observed in rats fed diets containing 0·25 and 0·5 % (w/w) α-lipoic acid were significantly higher than those in rats fed the diet free of α-lipoic acid. We also measured the activity of Gsr (Fig. 4(c)). Dietary α-lipoic acid dose dependently increased the activity of this enzyme. Consistent with the observation that α-lipoic acid increased the mRNA expression of proteins involved in the redox system, α-lipoic acid strongly and dose dependently reduced the concentrations of malondialdehyde, a marker of lipid peroxidation, in both the serum and liver (Fig. 4(d)).
Discussion
Previous studies have indicated that α-lipoic acid increases the mRNA expression or the activity or protein levels of enzymes involved in drug metabolism, including NAD(P)H:quinone oxidoreductase( Reference Jia, Hallur and Zhu 16 – Reference Ki and Kim 18 ), Gst-α2 and microsomal epoxide hydrolase( Reference Ki and Kim 18 ), in various types of cultured cells. However, an animal study examining the physiological activity of α-lipoic acid affecting drug-metabolising enzymes has been lacking.
The present study using DNA microarray analysis unequivocally demonstrated that dietary α-lipoic acid up-regulates the gene expression of various proteins involved in drug metabolism. Drug metabolism involves many enzymes that catalyse numerous types of chemical reactions, and each reaction is often catalysed by many isoenzymes differing in substrate specificity. Therefore, the DNA microarray technique is quite useful for identifying isoenzymes involved in drug metabolism specifically affected by various physiological and dietary factors.
The Cyp proteins are a superfamily of enzymes highly expressed in the liver and involved in the metabolism of xenobiotic compounds, as well as the synthesis and catabolism of endogenous compounds. Among the various Cyp, DNA microarray and real-time PCR analyses revealed that α-lipoic acid dose dependently increased the mRNA expression of Cyp4b1 and Cyp2b12. Cyp4b1 is involved in the ω-oxidation of lauric acid and mutagenic activation of some chemical compounds( Reference Imaoka, Yoneda and Matsuda 32 , Reference Imaoka, Hayashi and Hiroi 33 ). Some xenobiotic compounds, such as terephthalic acid, have been shown to increase the mRNA expression of Cyp4b1 in the liver( Reference Dai, Cui and Song 34 ), and caffeic acid has been shown to increase the mRNA expression in the colon( Reference Ye, Liu and Henderson 35 ). The role of Cyp2b12 in hepatic drug metabolism is not clear.
Fmo are another superfamily of enzymes involved in drug metabolism( Reference Krueger and Williams 36 ) and are expressed at high levels in the liver. Many different enzyme genes have been identified in mammals. Studies have indicated that Fmo1, Fmo3 and Fmo5 are the major Fmo in mouse liver and Fmo5 predominates over the other two isoforms( Reference Zhang, Cerny and Lawson 37 ). DNA microarray analysis revealed that the mRNA expression of Fmo5 but not of other Fmo was up-regulated by dietary α-lipoic acid. Some studies( Reference Zhang, Cerny and Lawson 37 , Reference Cherrington, Falls and Rose 38 ) have shown that Fmo5, similar to other Fmo, can oxidise various endogenous and xenobiotic substrates.
Many aldehydes generated during normal physiological processes are cytotoxic and carcinogenic. Aldh detoxify various aldehydes. Aldh is a superfamily consisting of many genes. In the present study, α-lipoic acid increased the mRNA expression of Aldh1a1, Aldh1a7 and Aldh18a1. Studies have indicated that Aldh1a1 is involved in the detoxification of various xenobiotic aldehydes( Reference Marchitti, Brocker and Stagos 39 ). As Aldh1a1 and Aldh1a7 appear to be coordinately regulated( Reference Alnouti and Klaassen 40 , Reference Tsuruoka, Kidokoro and Matsumoto 41 ), it is plausible that not only Aldh1a1 but also Aldh1a7 plays a crucial role in drug metabolism. The role of Aldh18a1 in drug metabolism is not clear at present.
The role of Nqo1 and Ephx1 in drug metabolism has been well documented( Reference Dinkova-Kostova and Talalay 42 , Reference Decker, Arand and Cronin 43 ). In the present study, we observed that α-lipoic acid increased the mRNA expression of these enzymes. This is agreement with the results of previous studies in cultured cells( Reference Jia, Hallur and Zhu 16 – Reference Ki and Kim 18 ).
It has been suggested that various Akr isoenzymes are involved in the detoxification of lipid aldehydes and various xenobiotic compounds( Reference Penning and Drury 44 ). DNA microarray and real-time PCR analyses revealed that α-lipoic acid dose dependently increased the mRNA expression of Akr7a3, Akr1d1 and Akr1c1. Akr7a3, alternatively known as aflatoxin aldehyde reductase, was discovered( Reference Ellis, Judah and Neal 45 ) as an enzyme to reduce aflatoxin B1-dihydrodiol to the dialcohol metabolite in rats. Studies( Reference Ellis, Judah and Neal 46 , Reference Kelly, Ellis and Manson 47 ) have demonstrated that this enzyme also reduces various aldehyde and keto substrates. In addition, studies( Reference Ellis, Judah and Neal 46 – Reference Wanichwatanadecha, Sirisrimangkorn and Kaewprag 48 ) have shown that many compounds having chemopreventive properties increase the expression of this enzyme. Studies have indicated that Akr1c1 plays a crucial role in the metabolism of xenobiotic compounds and in chemoprevention( Reference Jin, Mesaros and Blair 49 ). Akr1d1 may play a crucial role in bile acid synthesis( Reference Chen, Drury and Penning 50 ) rather than in drug metabolism. Data suggest that several Akr isoforms convert polycyclic aromatic hydrocarbons into carcinogenic compounds, referred to as remote quinones( Reference Shultz, Quinn and Park 51 ). This does not comply with the consideration that Akr are involved in chemoprevention.
Carboxylesterases comprise a superfamily of microsomal enzymes that catalyse the hydrolysis of a variety of ester- and amide-containing chemicals to their respective free acids. They are involved in the detoxification or metabolic activation of xenobiotic compounds( Reference Satoh and Hosokawa 52 ). Dietary α-lipoic acid increased the mRNA expression of Ces2c but not of other isoenzymes. Ces2 isoforms can hydrolyse various xenobiotic compounds( Reference Satoh and Hosokawa 52 ). Therefore, the increase in the mRNA expression of a member of the Ces2 family may stimulate the metabolism of xenobiotic compounds.
More than twenty Gst isoenzymes have so far been identified in rats. In spite of the fact that the DNA microarray contained nineteen probes for various Gst, we observed that the diet containing 0·5 % (w/w) α-lipoic acid significantly increased the mRNA expression of Gsta3, Gstt1 and Gstt3, Gstp1 and Gsto1 but not of other Gst more than 1·5-fold. Therefore, the effect of α-lipoic acid on the mRNA expression of Gst was again isoenzyme specific. It has been reported that several synthetic or natural compounds with anti-carcinogenic activities increase the mRNA or protein expression of Gsta3 and Gstp1 in rat liver( Reference Kelly, Ellis and Manson 47 , Reference Primiano, Egner and Sutter 53 ). So, it is possible that these isoforms play a role in the detoxification of xenobiotic compounds and cancer prevention. Also, some epidemiological surveys have indicated that GSTT1 deletion in humans increases the risk of cancer( Reference Josephy 54 ). Gstt3 has so far been identified in mice and rats and is highly expressed in the liver( Reference Coggan, Flanagan and Parker 55 ). However, the physiological significance of this Gst isoenzyme in detoxification and cancer prevention is not known. Gsto1 is expressed abundantly in the liver, macrophages, and glial and endocrine cells( Reference Luo, Kinsey and Schiffman 56 ), but information regarding the role of this isoform in drug metabolism is scarce. A case–control study failed to find a clear-cut relationship between GSTO1 polymorphisms and cancer risk( Reference Beebe-Dimmer, Iyer and Nriagu 57 ). We observed that dietary α-lipoic acid increased cytosolic Gst activity when using 1-chloro-2,4-dinitrobenzene and 1,2-dichloro-4-nitrobenzene as substrates. However, the extent of the increases was much lower than that observed for the mRNA levels of Gsta3, Gstt1 and Gstt3, Gstp1 and Gsto1. This is not surprising because the effect of α-lipoic acid on Gst was isoenzyme specific and it did not affect the mRNA levels of many other Gst. α-Lipoic acid failed to affect enzyme activity when using p-nitrobenzyl chloride and ethacrynic acid as substrates. The substrate specificity of each Gst isoenzyme differs considerably( Reference Luo, Kinsey and Schiffman 56 ). Therefore, it is reasonable that α-lipoic acid did not increase the amount of Gst molecules, which is specific to p-nitrobenzyl chloride and ethacrynic acid.
Cytosolic Sult are phase II drug-metabolising enzymes. In mammals, four to five gene families of Sult have been identified( Reference Gamage, Barnett and Hempel 58 ). Each family comprises more than one member, and the DNA microarray used in the present study contained seven probes for various Sult1 family members, five for Sult2 family members, and one each for Sult4 and Sult5 members. Among the various Sult, α-lipoic acid increased the mRNA expression of Sult1c2, but not of the other isoforms. It has been reported that phenolic compounds including carcinogens can serve as substrates for Sult belonging to the 1c family( Reference Gamage, Barnett and Hempel 58 ).
Among the various Ugt isoenzymes, α-lipoic acid significantly increased the mRNA expression of UDP glucuronosyltransferase 2 family, polypeptide B17 (Ugt2b17) and isoenzyme(s) belonging to the Ugt1a family. Ugt belonging to 1a and 2b families are abundantly expressed in the liver and catalyse the glucuronidation of various endogenous and xenobiotic compounds( Reference Bock 59 ).
The Abc transporters transport a wide variety of exogenous and endogenous substances across membranes. There are seven subfamilies, termed Abca, Abcb, Abcc, Abcd, Abce, Abcf and Abcg. Many Abc transporters are involved in the export of xenobiotic compounds and hence in drug resistance. In the present study, α-lipoic acid increased the mRNA expression of three Abc transporters (one each from Abca, Abcb and Abcc subfamilies). As these Abc subfamilies play crucial roles in the export of xenobiotics out of the cell( Reference Dean, Hamon and Chimini 60 ), α-lipoic acid may stimulate drug metabolism through the up-regulation of not only phase I and II enzymes but also phase III transporters.
α-Lipoic acid increased the mRNA expression of Nr1i3, alternatively known as constitutive androstane/activated receptor (Car). This transcription factor activates various genes involved in drug metabolism( Reference Tolson and Wang 28 ). Therefore, up-regulation of the mRNA expression of this transcription factor may account for the α-lipoic acid-dependent increase in the mRNA levels of various proteins involved in drug metabolism.
In the present study, we demonstrated that α-lipoic acid increases the gene expression of proteins involved in the antioxidation system in addition to that of those involved in drug metabolism. The observations that α-lipoic acid increased hepatic glutathione concentration and mRNA levels of two subunits of γ-glutamylcysteine ligase (Gclc and Gclm) were in agreement with those made by Suh et al. ( Reference Suh, Shenvi and Dixon 61 ). Xu et al. ( Reference Xu, Gao and Song 8 ) have also recently reported that α-lipoic acid increases hepatic glutathione concentration and activities of enzymes involved in the antioxidation system. Moreover, in the present study using DNA microarray analysis, we demonstrated that α-lipoic acid increases the mRNA expression of various other proteins presumed to be involved in the thiol redox system, including Srxn1, Gpx2, Apex1, Txnrd1, Gsr and Glrx2 (cytosolic form of Glrx), but decreases that of the mitochondrial form of Glrx (Glrx1). However, real-time PCR analysis indicated that α-lipoic acid is rather weak in terms of affecting the mRNA expression of Glrx1. In addition to the proteins involved in the thiol redox system, α-lipoic acid significantly increased the mRNA expression of metallothioneins (Mt1a and Mt2A). Studies have indicated that metallothionein plays a crucial role in the prevention of oxidative stress in animals( Reference Swindell 29 ). Haeme oxygenase is involved in the conversion of haeme into strong antioxidants (biliverdin and biliverdin)( Reference Wu, Ho and Lin 62 ). Therefore, haeme oxygenase is considered to play a decisive role in the attenuation of the oxidative process. So far, two forms of haeme oxygenase (Hmox1 and Hmox2) have been identified in both humans and rodents. Hmox1 but not Hmox2 is considered to play a crucial role in protection against oxidative stress( Reference Wu, Ho and Lin 62 ).
Some previous studies( Reference Suh, Shenvi and Dixon 61 , Reference Jung, Kim and Shin 63 , Reference Castro, Massa and Schinella 64 ) have indicated that α-lipoic acid increases the expression of genes involved in the antioxidation system. The present study extended this evidence and newly identified many genes involved in the antioxidation system that are affected by α-lipoic acid. Therefore, it is plausible that this at least partly accounts for the potent antioxidation activity of dietary α-lipoic acid, as confirmed in the present study using malondialdehyde as a marker of lipid peroxidation.
A transcription factor called nuclear factor, erythroid derived 2, like 2 (Nfe2l2) or NFE2-related factor 2 (Nrf2) regulates the gene expression of many enzymes involved in the antioxidation system and drug metabolism( Reference Suh, Shenvi and Dixon 61 , Reference Klaassen and Reisman 65 ). There is a possibility that this transcription factor is involved in α-lipoic acid-dependent changes in the mRNA expression of proteins involved in drug metabolism and the antioxidation system. In fact, the mRNA expression of many genes targeted by this transcription factor, such as Nqo1, Hmox1, subunits of glutamate–cysteine ligase (Gclm and Gclc), Ephx1, Srxn1 and Abcc4, was up-regulated by dietary α-lipoic acid. Moreover, recent studies have indicated that Nrf2 is also involved in the regulation of hepatic lipid biosynthesis( Reference Vomhof-Dekrey and Picklo 66 ). Therefore, alterations in the Nrf2 signalling pathway may account for not only the α-lipoic acid-dependent changes in the mRNA expression of proteins involved in drug metabolism and the antioxidation system observed in the present study, but also the reduction in lipid biosynthesis reported previously( Reference Huong and Ide 12 – Reference Ide, Azechi and Kitade 14 ).
Finlay et al. ( Reference Finlay, Michels and Butler 67 ) have recently reported the results of DNA microarray analysis on the hepatic gene expression of young and old rats fed α-lipoic acid. Consistent with our previous studies( Reference Huong and Ide 12 – Reference Ide, Azechi and Kitade 14 ) and the present study, they found that α-lipoic acid strongly reduced the mRNA levels of proteins involved in lipogenesis. They also suggested that α-lipoic acid altered the expression of genes governing circadian rhythm. However, they did not make any comment regarding the effect of α-lipoic acid on proteins involved in drug metabolism and in the antioxidation system.
Previous animal experiments( Reference Xu, Gao and Song 8 – Reference Ford, Cotter and Cameron 11 , Reference Jung, Kim and Shin 63 ) using rats or mice have employed dietary levels of α-lipoic acid of 0·05–1 % (w/w), which are similar to the levels employed in the present study. A nutritional survey conducted in the UK in 2008–9( Reference Whitton, Nicholson and Roberts 68 ) has indicated the median food intake of adult humans to be 435 and 338 g/d for men and women, respectively. A nutritional survey conducted in Japan in 2011 (http://www.mhlw.go.jp/stf/houdou/2r9852000002q1st-att/2r9852000002q1wo.pdf) has also indicated the average food intake of adult humans to be 447 and 374 g/d for men and women, respectively. Therefore, the intake of diets containing 0·1, 0·25 and 0·5 % (w/w) α-lipoic acid used in the present animal study corresponds to the daily consumption of approximately 340–450, 850–1100 and 1700–2200 mg/person of this compound, respectively, when extrapolated to humans. These values are comparable to those employed in previous human studies (200–2400 mg/d per person)( Reference Wollin and Jones 2 ). With regard to the safe dose level of α-lipoic acid, the acute LD50 (lethal dose 50 %) appeared to be very high in rats (>2000 mg/kg body weight), although lower values have been reported in some other species (dogs, mice and cats) and the NOAEL (no observed adverse effect level) has been estimated to be 61·9 mg α-lipoic acid/kg body weight per d for rats( Reference Wollin and Jones 2 ). On the basis of the body weight and food intake of rats observed in the present study, approximate dose levels of α-lipoic acid were estimated to be 16, 40 and 80 mg/kg body weight per d for animals fed diets containing this compound at the levels of 0·1, 0·25 and 0·5 % (w/w), respectively. Therefore, these values did not markedly exceed the NOAEL of α-lipoic acid, although dietary levels of 0·25 and 0·5 % (w/w) significantly reduced the body weight of animals. The diet containing 0·25 % (w/w) α-lipoic acid reduced the growth of rats without significantly affecting food intake in the present study. In this context, it has been reported that α-lipoic acid increases energy expenditure( Reference Kim, Park and Namkoong 69 , Reference Wang, Li and Guo 70 ) and reduces intestinal sugar absorption( Reference Prieto-Hontoria, Pérez-Matute and Fernández-Galilea 71 ) in rats.
It has been reported that orally administered α-lipoic acid in rats is well absorbed from the intestine( Reference Wollin and Jones 2 , Reference Peter and Borbe 72 ). Pharmacokinetic analyses of the metabolic fate of orally and intravenously administered radiolabelled α-lipoic acid have indicated that 66 % of orally administered α-lipoic acid is absorbed from the intestine. An alternative evaluation based on the measurements of urinary excretion of 14C gave a higher value of absorption (93 %)( Reference Peter and Borbe 72 ).
In conclusion, DNA microarray and real-time PCR analyses revealed that dietary α-lipoic acid strongly increases the mRNA expression of various proteins involved in drug metabolism and the antioxidation system. Therefore, it is expected that α-lipoic acid would be effective at ameliorating pathological conditions induced by physiological factors and xenobiotic toxic compounds. In this context, it has been well demonstrated that compounds having the propensity to increase the activity and gene expression of enzymes involved in drug metabolism exhibit chemopreventive effects. In fact, some studies have indicated that α-lipoic acid is effective against tumour development( Reference Schwartz, Guais and Israël 73 ). Evaluation of the physiological effect of α-lipoic acid in pathological conditions would clarify the physiological significance of the up-regulation of the gene expression of proteins involved in drug metabolism and antioxidation by α-lipoic acid. This needs to be clarified in future studies.
Acknowledgements
The present study was supported by a grant-in-aid for scientific research (Scientific Research C, no. 22580143) from the Japan Society for the Promotion of Science and a grant from the Ministry of Agriculture, Forestry, and Fisheries research project ‘Development of evaluation and management methods for supply of safe, reliable and functional food and farm produce’.
The author's contributions are as follows: T. I. designed and carried out the animal experiment, analysed the data and prepared the manuscript.
The author declares no conflicts of interest.