Differential Roles of Peroxisome Proliferator-Activated Receptor-α and Receptor-γ on Renal Crystal Formation in Hyperoxaluric Rodents

Peroxisome proliferator-activated receptors (PPARs) and related inflammatory and oxidative molecule expression were investigated in a hyperoxaluric rodent model to evaluate the in vivo efficacy of PPAR agonists in preventing renal crystal formation. PPAR expression was examined in a mouse hyperoxaluria kidney stone model induced by daily intra-abdominal glyoxylate injection. Therapeutic effects of the PPARα agonist fenofibrate and PPARγ agonist pioglitazone were also assessed in a 1% ethylene glycol-induced rat model of hyperoxaluria. Crystal formation, inflammation, cell injury, apoptosis, and oxidative stress were compared to those of vehicle-treated controls. Quantitative reverse transcription-polymerase chain reaction revealed that PPARα and PPARγ expression decrease and increase, respectively, during crystal formation in hyperoxaluric kidneys. In addition, PPARα localized to the cytoplasm of both proximal and distal tubular cells, whereas PPARγ accumulated in the nucleus of proximal tubular cells. Furthermore, renal crystal formation was significantly less prevalent in pioglitazone-treated rats but higher in the fenofibrate-treated and fenofibrate/pioglitazone-cotreated groups compared to controls, thus indicating that pioglitazone, but not fenofibrate, markedly decreased cell inflammation, oxidative stress, and apoptosis. Collectively, the results demonstrated that PPARγ suppressed renal crystal formation via its antioxidative and anti-inflammatory effects; however, the renotoxicity of PPARα may elicit the opposite effect.


Introduction
Kidney stone disease has lifetime prevalence and recurrence rates nearing 10% and 50%, respectively [1], and is associated with development of end stage renal disease and cardiovascular disease [2,3]. Recent studies have demonstrated that obesity, inflammation, and oxidative stress-related characteristics similar to metabolic syndrome (MetS) potentiate kidney disease [4]. Moreover, evidence suggests that obesity, weight gain, and high-calorie diets increase the kidney stone formation risk by 1.5-2.0-fold [5]. The estimated annual cost of treatment for kidney stones in the US will rise approximately 1.2-fold to 4.6 billion dollars in 2030 due to the increasing incidence of MetS in the population [6]; thus, a novel preventive therapy is needed to reduce potential burden to the economy and healthcare system.
Kidney stones are hypothesized to form from crystal nidi, which grow, aggregate, and subsequently obstruct the tubular lumen [7]. Numerous studies in hyperoxaluric rat and mouse models induced by ethylene glycol (EG) [8,9] and glyoxylate (GOX) administration show that renal crystal formation is enhanced by oxidative stress generated in response to ROS and proinflammatory chemokines and cytokines [7,10]. In addition, the expression of various adipocytokines-such as interleukin-6 (IL-6), monocyte chemotactic protein-1 (MCP-1), and adiponectin (APN)-promotes crystal formation by 2 PPAR Research elevating OPN expression, which associates with the calcium oxalate (CaOx) stone matrix in MetS [11].
Although statins and PPAR agonists are often used to treat MetS-related disease, there is currently no therapy designed to target the molecular mechanism underlying renal crystal formation. PPARs are intranuclear receptors that induce peroxisome proliferation, control gene expression related to hydrocarbons, lipids, and protein metabolism, and facilitate cell differentiation [12]. More specifically, PPAR regulates lipid metabolism by targeting fatty acid and acyl-CoA and thus acts as protective factor in dyslipidemia, whereas PPAR increases tissue insulin sensitivity and is a pharmaceutical target in diabetes mellitus. Notably, both PPAR and PPAR agonists reportedly exhibit renoprotective functions through their anti-inflammatory and oxidative effects [13,14]; however, some studies have published that PPAR agonists show differential effects on oxidative stress and renal function [15,16].
Therefore, we sought to evaluate the in vivo efficacy of PPAR / agonists in preventing renal crystal formation and investigated the changes in expression of PPARs and other inflammatory and oxidative stress-related molecules in hyperoxaluric animal models.

Animal Procedures.
All experimental procedures were performed according to the National Institutes of Health's Guide for the Care and Use of Laboratory Animals, and the procedures were approved by the Animal Care and Use Committee of the Faculty of Medicine, Nagoya City University Graduate School of Medical Sciences.
Male C57BL/6J mice were purchased from Charles River Japan (Yokohama, Japan). The mice were fed with standard chow (MEQ, containing 1.01 g/100 g calcium, 0.78 g/100 g phosphorus, and 0.21 g/100 g magnesium; Oriental Yeast Co., Tokyo, Japan) and had free access to water. Based on our previous report [17], 8-week-old mice were given daily intraabdominal injections of 80 mg/kg GOX; the kidneys were extracted on days 0, 3, 6, 9, and 12 ( = 6 per group) to examine crystal formation and PPAR gene expression.
Eight-week-old male Sprague-Dawley rats (Japan SLC Inc., Shizuoka, Japan) were divided into five groups ( = 6/group) to assess the effects of the PPAR and PPAR agonists, fenofibrate (FF), and pioglitazone (PGZ), respectively. Animals had access to standard chow (CE-2, containing 1.06 g/100 g calcium, 0.99 g/100 g phosphorus, and 0.34 g/100 g magnesium; CLEA Japan Inc., Tokyo, Japan) throughout the experiment. Animals were left untreated (control group) or treated with 1% EG (EG group), 1% EG and 30 mg/kg FF (EG + group), 1% EG and 10 mg/kg PGZ (EG + group), or 1% EG and 30 mg/kg FF and 10 mg/kg PGZ (EG + group). FF and PGZ were administered via the gastric tube as described previously [18,19]. Blood and 24 h urine samples and kidney sections were collected on day 14 ( = 6 per group). Blood and urinary biochemistry were analyzed by LSI Medience Corporation, Tokyo, Japan. Urinary pH and volumes were measured manually. Urinary oxalate concentrations were analyzed using a chemiluminescence analyzer (FOM-110A; Hokuto Denko Corporation, Tokyo, Japan).

Observation of Renal CaOx Crystals.
Extracted kidneys were examined for crystal formation by Pizzolato staining and polarized light optical microphotography. Cross sections (4-m) were stained with Pizzolato according to a previously described method for oxalate-containing crystal detection [20]. Crystal formation was qualitatively assessed in nonstained kidney sections by using polarized light optical microphotography and quantitatively assessed using Image Pro Plus (Media Cybernetics, Inc., Rockville, MD).

Immunohistochemistry of PPARs, Inflammation-Related,
and Oxidative Stress-Related Genes. PPAR and PPAR expression were analyzed by immunohistochemical staining of 4 m-thick cross sections of mice kidneys. Anti-mouse PPAR rabbit polyclonal antibody (Abcam, Inc., Cambridge, MA) and anti-mouse PPAR rabbit monoclonal antibody (Cell Signaling Technology, Inc., Danvers, MA) were used as primary antibodies at concentrations of 5 g/mL and 1.5 g/mL, respectively. Immunoreactivity was detected using a Histofine Simple Stain Kit for rabbit IgG (Nichirei Biosciences, Inc., Tokyo, Japan).

Evaluation of Apoptosis.
TUNEL assays were performed to detect apoptotic renal tubular cells by using an in situ cell death detection kit (Roche Applied Science, Indianapolis, IN). The number of TUNEL-positive cells was counted in 20 different fields for each section under ×400 magnification.

Statistical Analysis.
All data are expressed as mean ± standard error. The statistical analyses were performed using a two-way ANOVA for comparisons among three or more groups, or the Mann-Whitney test for comparisons between two groups. All statistical analyses were performed using Statistical Analysis System, version 9.1 (SAS Institute Inc., Cary, NC). values < 0.05 were considered statistically significant.

Renal CaOx Crystal Deposits and PPAR Expression in
Hyperoxaluric Mice. To clarify the roles of PPAR and PPAR in kidney stone formation, we first examined their expression using hyperoxaluric stone model mice. Renal crystal deposits were detected after 3 days of GOX administration, peaked on day 6, and disappeared by day 12 (Figure 1(a)), consistent with previous reports [12]. PPAR mRNA expression analysis in renal tissue from GOX-treated mice showed an increase in transcript expression on day 6, which is in direct contrast to the lower PPAR observed on day 6 ( Figure 1(b)).
Moreover, CaOx deposits detected by Pizzolato staining were localized to the intratubular space at the corticomedullary junction of mouse kidneys. Strong PPAR staining was observed in the cytoplasm of both proximal and distal tubules, particularly in day 0 controls, whereas PPAR was detected in nucleus of proximal tubular cells, but not in the tubular cells affected by CaOx crystals (Figure 1(c)).

Observation of Renal CaOx Crystals in Hyperoxaluric
Rats Treated with PPAR Agonists. Intratubular CaOx crystal deposits developed in the corticomedullary lesion of rat kidneys after 14 days of EG administration, as detected by Pizzolato staining (Figure 2(a)). Notably, larger renal crystal deposits were observed in the EG + and EG + groups and smaller amounts were found in the EG + group than in the EG and control groups. No significant difference in crystal deposits rates was found between the EG + and EG + groups (Figure 2(b)).

Physical, Serum, and Urinary
Variables. The body weight of the EG + and EG + groups was significantly lower than that in the control and EG groups, while body weight of the EG + group was lower than that of the control group but did not differ from that of the EG group. In addition, kidney weights in the EG, EG + , and EG + groups were markedly higher than that of controls, whereas these were significantly lower in the EG + group than in the EG group (Table 1).
In terms of serum biochemistry, creatinine and phosphorus levels were significantly higher in EG + and EG + rats than in their control and EG counterparts. No statistical differences were found among the five groups with respect to serum calcium or triglyceride levels, except for the EG group. Furthermore, serum blood sugar concentrations were lower in the EG + and EG + groups than in others, while total cholesterol concentrations were lower in the EG + and EG + groups. (Table 1) Urinary volume and oxalate excretion were markedly higher in all EG-treated groups, whereas calcium excretion was lower than that in the control group. No statistical differences were found in urinary pH or phosphorus excretion across all treatment groups (Table 1).

PPAR and PPAR Expression in Hyperoxaluric Rats.
PPAR mRNA expression was lower in the EG, EG + , and EG + groups than that in the control group. Particularly, mRNA expression of PPAR was the lowest in the EG + and EG + . PPAR mRNA expression was lower in all EGtreated groups than that in the control group; however, there were no significant differences among them (Figure 3(a)).
On the contrary, PPAR and PPAR protein expression were higher in the EG + and EG + groups when compared with the other groups, respectively (Figure 3(b)).

Proinflammatory-Related Gene
Expressions. The macrophage proinflammatory proteins OPN, MCP-1, and ED1 were strongly detected in the corticomedullary region of EG, EG + , and EG + rat kidneys (Figure 4(a)). OPN was observed in inner tubule side of renal proximal tubular cells, whereas MCP-1 was observed in intracellular space of both renal tubular and interstitial cells. ED1-positive cells localized to the peritubular and interstitial space around crystal deposits. In the EG + group, MCP-1 and ED1 expression was weak when compared to the EG, EG + , and EG + groups. In qRT-PCR analyses, Spp1 and Cd68 were highly expressed in the EG, EG + , and EG + groups than in the control group, with expression in the EG + group notably higher than that in the EG and EG + groups. Ccl2 expression   Crystallization in each kidney section was quantified by calculating the ratio (%) of the area with crystals to that of the entire kidney section by using Image Pro Plus ( = 6 for all groups). Data are presented as mean ± SE. * < 0.05 among EG + , EG + , and EG + groups; † < 0.05 compared with the control group; § < 0.05 compared with the EG group. Data of control, EG, and EG + groups obtained by our previous study [26].   in the EG + group was markedly higher than that in the control and EG + groups (Figure 4(b)).

Anti-Inflammatory and Oxidative Stress Gene Expression.
APN and SOD1 immunostaining demonstrated reduced expression in the EG, EG + , and EG + groups than in the control and EG + groups, which localized to renal tubular cells in the corticomedullary and medullary space ( Figure 5(a)).
By qRT-PCR, Adipoq and Sod1 expression in the EG + group were significantly lower than those in the control and EG + groups. Adipoq expression in the EG + group was also lower than that in the EG group ( Figure 5(b)).

Evaluation of Cellular
Apoptosis. TUNEL-positive cells were observed within the renal proximal tubule mostly localized around crystal deposits and the glomerulus in EGtreated kidneys (Figure 6(a)). The number of TUNEL-positive cells in the EG, EG + , and EG + groups was significantly higher than in the control and EG + groups (Figure 6(b)).
Procaspase-9 expression was high in the EG and EG + groups, whereas cleaved caspase-9 cleavage fragments were highly detected in the EG + and EG + when compared to other groups. In addition, caspase-3 expression was markedly higher in the EG, EG + , and EG + groups than the other groups ( Figure 6(c)).

Discussion
PPARs are transcription factors that regulate gene expression related to effects of intracellular lipids and inflammatory mediators. Although the exact role of PPARs in kidney stone pathogenesis is yet unknown, we revealed that PPAR and PPAR exhibit differential effects on this process in hyperoxaluric mice and rats. More specifically, GOX-treated mice showed renal CaOx crystal depositions on days 3 and 6, which decreased by day 9. Interestingly, the expression of these PPARs was different-with lower PPAR expression and higher PPAR expression during renal crystal formation. Additionally, PPAR localized within the tubular cytoplasm among proximal and distal tubules and collecting ducts, whereas PPAR was observed in the nucleus of proximal tubules as previously reported [21], but not in crystal-induced injured tubules. These findings are indicative of sufficient, and possibly heightened, PPAR expression in renal tubular cells; however, PPAR expression was specifically found in the tubules in the cortex under a normal physiological state. Moreover, CaOx crystal development decreased PPAR expression throughout the kidney but increased PPAR expression in healthy tubular cells that were undamaged by crystal deposits.
Based on results from the experimental rat model, we identified that the two PPAR agonists have differential effects on kidney stone formation: PGZ and FF attenuated and Scale bar = 100 m. (b) Gene expression was measured by qRT-PCR using TaqMan assays ( = 6 for all groups). Data are presented as the mean ± SE. * < 0.05 among EG + , EG + , and EG + groups; † < 0.05 compared with the control group; § < 0.05 compared to the EG group. accelerated EG-induced crystal development, respectively. With regard to urinary mineral excretion, no significant differences were observed among EG, EG + , EG + , and EG + groups. Since rats generally prefer to drink EG over water, all EG-treated groups had higher urine volume compared to the control group. Moreover, the urinary calcium excretions in all EG-treated rats were lower than those in controls because of the formation of renal CaOx crystals [22]. These results support known evidence that PGZ and FF do not interfere with urinary parameters that affect renal crystal development.
PPAR agonists, such as PGZ, have anti-inflammatory and antioxidative effects. PGZ treatment suppressed inflammatory-related gene expression including that of OPN, MCP-1, and ED1, the number of TUNEL-positive apoptotic cells, and caspase-9 and caspase-3 expression, whereas these were increased in FF-treated rats. FF rats showed decreased APN and Sod1 expression, which are considered anti-inflammatory and antioxidative molecules. Kidney stone formation results from reactive oxygen species (ROS) production, which is facilitated by inflammatory molecules and macrophage infiltration [23]. Consistently, metabolic disorders accelerate the stone development via inflammatory adipocytokines, which is hindered by APN expression [24,25].
Some reports, including our previous study, have suggested that PGZ suppressed renal crystal formation as well as acute renal injury by inhibiting cellular inflammation, ROS production, and apoptosis in rat models [13,26]. Mechanistically, FF binds to and activates PPAR , thereby reducing fasting triglyceride and low-density cholesterol levels in blood plasma. In addition, Frazier-Wood and colleagues reported that FF treatment increased serum MCP-1 but decreased serum APN concentrations during a single nucleotide polymorphism study of human PPAR [27]. . Data are presented as mean ± SE. * < 0.05 among EG + , EG + , and EG + groups; † < 0.05 compared to the control group; § < 0.05 compared to the EG group. (c) Western blotting of rat kidneys for caspase-9 and caspase-3 protein levels. The molecular mass of procaspase-9, cleaved caspase-9, and caspase-3 was confirmed by bands at 51, 37, and 35 kDa, respectively.
In this study, treatment with PPAR agonist suppressed body weight gain in rats. EG and FF treatment enlarged the rat's kidney, and FF increased the serum level of creatinine, which is likely the result of FF-induced renotoxicity, particularly during the early phrase of treatment. Patients with older age, of male gender, with high serum creatinine, and using high doses of FF are considered at high risk for adverse effects. FF is hypothesized to reduce the renal blood flow by affecting the expression of vasodilatory prostaglandins [28]. Stoller and colleagues insisted that kidney stone development is caused by renovascular flow dysfunction [29]. We used 30 mg⋅kg −1 ⋅day −1 of FF for rat, which was 10 times higher than the human dose of 3 mg⋅kg −1 ⋅day −1 . Besides, these "male" rats already had the relative serum creatinine elevation and crystal-induced tubular cell injury. As such, the adverse effects of high-dose FF and crystal-induced renotoxicity may further accelerate crystal deposit formation and renal dysfunction.
Despite promising results, our study is limited by the dissimilarities between the various animal models of kidney stone development. It has two primary limitations. For instance, rodent stone models develop acute and excessive renal crystal deposits compared to humans; however, similarities between the mechanisms of intratubular crystal formation make these models suitable for translational research on renal disease. Additionally, the doses of PPAR agonists given to rats in our study were relatively higher than those used in humans; however, our results on PPAR and PPAR renal expression showed that appropriate drug delivery should be investigated further. Further pharmacokinetics studies are needed to clarify the significance of our results.

Conclusions
Collectively, we established the differential effects of PPAR agonists on renal crystal formation, where PPAR and PPAR convey renotoxic and renoprotective effects, respectively, in the hyperoxaluric kidney environment. Since PPAR and PPAR are differentially expressed in the kidneys, it is reasonable that these two effectors play opposing roles in tubular cell CaOx crystal deposition and should be considered when treating MetS patients with kidney stones.