Retraction Note: pNaKtide Attenuates Steatohepatitis and Atherosclerosis by Blocking Na/K-ATPase/ROS Amplification in C57Bl6 and ApoE Knockout Mice Fed a Western Diet

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Effect of pNaKtide on fatty acid oxidation genes in adipose tissue of mice fed a western diet. Since adipose mitochondria participate in energy expenditure through fatty acid oxidation, quantitative PCR was done to measure fatty acid oxidation genes in adipose tissue. Peroxisome proliferator-activated receptor gamma coactivator 1-alpha (PGC-1α) is a major regulator of mitochondrial oxidative metabolism 22 . Our results showed that PGC-1α mRNA expression was significantly decreased in adipose tissue of C57Bl6 or ApoE−/− mice fed a western diet compared to the control group ( Table 2). Administration of pNaKtide significantly increased PGC-1α mRNA expression in these mice. Carnitinepalmitoyltransferase-1 (CPT-1) is a rate-limiting enzyme of mitochondrial fatty acid β-oxidation 23 . CPT-1 mRNA expression was decreased in both C57Bl6 and ApoE−/− mice fed a western diet compared to control mice and this decrease was reversed by treatment with pNaKtide ( Table 2). The UCP 1 and 2 are markers of energy metabolism and its uncoupled energy is used for heat production in fat tissue 24 . Our results demonstrated that both strains of mice fed a western diet exhibited decreased expression of UCP 1 and 2 in adipose tissue in comparison to mice fed a normal diet. Our results showed that UCP1 and 2 mRNA expressions were significantly increased by pNaKtide treatment in adipose tissue compared to mice fed a western diet in both strains of mice ( Table 2).
Effect of pNaKtide on hepatic lipogenesis and inflammation in mice fed a western diet. Histological sections of liver tissue from C57Bl6 mice fed a western diet showed significant inflammation and a large number of vacuoles in the liver. C57Bl6 mice treated with pNaKtide exhibited decreased lipid and inflammatory cell infiltration as seen by H&E staining (Fig. 1A). H&E staining of liver tissues from ApoE−/− mice fed a western diet also had a significant increase in lipid and inflammatory cell infiltration compared to control ApoE−/− mice. pNaKtide decreased lipid and inflammatory cell infiltration compared to mice fed a western diet (Fig. 1B). Both C57Bl6 and ApoE−/− mice fed a western diet had significantly increased lipid accumulation in the liver compared to mice fed a normal chow diet (Fig. 1C,D) as demonstrated by Oil red O staining and administration of pNaKtide decreased this. Increased fat accumulation in hepatocytes is mostly attributed to enhanced uptake and synthesis of fatty acids and triglycerides 25 . Our results showed that hepatic triglycerides and FFA levels were significantly increased in C57Bl6 and ApoE−/− mice fed a western diet compared to control mice ( Table 3). As expected, pNaKtide treatment significantly decreased hepatic triglycerides and FFA levels compared to mice fed a western diet.
Fatty acid synthase (FAS) expression, an important marker of lipogenesis, was increased in both strains of mice fed a western diet and this elevated level was decreased to control levels with pNaKtide treatment (Table 3). CD36, a fatty acid transport protein, contributes to the progression of inflammation in NASH 5,26 . Our results showed that CD36 mRNA expression was significantly increased in both strains of mice fed a western diet compared to control mice, and this increase was negated by treatment with pNaKtide (Table 3). Similarly, F4/80, MCP-1 and IL-6 mRNA expression, markers of macrophage/kupffer cell infiltration and inflammation 27 , were also increased in both strains of mice fed a western diet compared to control mice (Table 3). These changes were significantly attenuated with pNaKtide treatment.
Effect of pNaKtide on hepatic fibrosis in mice fed a western diet. Masson's trichrome staining of liver sections from both strains of mice fed a western diet demonstrated focal portal fibrosis (blue staining) compared to control mice and this increase was negated by treatment with pNaKtide ( Fig. S3A,B). Excess collagen synthesis in the liver is a sensitive indicator of NASH and fibrosis 28 . Type 1-collagen levels were significantly increased in both strains of mice fed a western diet, and this was significantly decreased to control levels with pNaKtide treatment (Fig. S3C,D). Similarly, mRNA expression of hepatic fibronectin, MMP9 and MMP13, genes related to fibrogenesis 29,30 , were also elevated in both strains of mice fed a western diet, and these increases were also attenuated with pNaKtide treatment ( Table 3).
Effect of pNaKtide on hepatic p-Src, ERK, and α1 carbonylation in mice fed a western diet. Protein carbonyl groups are widely used markers for oxidative stress 15 . We have shown previously that reactive oxygen species (ROS) initiates carbonylation of the α1 Na/K-ATPase subunit which in turn activates the Src signaling cascade with downstream modulation of extracellular signal-regulated kinase 1/2 (ERK1/2) 20 . Our results showed that carbonylation of the α1 Na/K-ATPase subunit was increased in C57Bl6 and ApoE−/− mice fed a western diet, and this increase was negated by pNaKtide treatment ( Fig. 2A and B). Treatment with pNaKtide also blocked Na/K-ATPase-regulated Src and ERK 1/2 activation in both strains of mice fed a western diet ( Fig. 2C-F). Further our results showed that TBARS, another marker of oxidative stress, was decreased by pNa-Ktide treatment compared to mice fed a western diet (Table 3), demonstrating pNaKtide-mediated abrogation of NASH and oxidative stress.
Effect of pNaKtide on hepatic mitochondrial fatty acid oxidation in mice fed a western diet. Mitochondria play an important role in energy metabolism, being the primary site for fatty acid oxidation in the liver [31][32][33] . Our results showed that hepatic PGC1α levels were decreased in both strains of mice fed a western diet compared to the control groups, and pNaKtide treatment significantly increased hepatic PCG1α expression ( Fig. 3A and B). In the mitochondrial extract of both mice strains fed a western diet, the hepatic expression of CPT-1 was less compared to the control group ( Fig. 3C and D). Administration of pNaKtide increased CPT-1 levels significantly compared to mice fed a western diet. Long-chain acyl-CoA dehydrogenase (LCAD), is involved in the first reaction of mitochondrial fatty acid oxidation and is important for energy homeostasis 23 . Similar to previous studies 34,35 , our results demonstrated that LCAD levels were significantly increased by pNaKtide treatment in liver mitochondrial extracts compared to mice fed a western diet ( Fig. 3E and F). Quantitative PCR was also done for the above genes and our results followed the same trend as the Western blot analysis. As expected, PCG1α, CPT-1 and LCAD mRNA expression were significantly increased by pNaKtide treatment in both C57Bl6 and ApoE−/− mice fed a western diet ( Table 3).
Effect of pNaKtide on metabolic profile in mice fed a western diet. The insulin resistance phenotype in both strains of mice fed a western diet was reversed by the administration of pNaKtide. This was

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characterized by improved glucose tolerance (Fig. 4) and a significant improvement in the homeostasis model assessment of insulin resistance (HOMA-IR) score (Table 4). Increased plasma ALT, FFA and triglycerides levels are strongly associated with insulin resistance and NASH. The administration of pNaKtide significantly attenuated the diet induced increase in plasma ALT, triglyceride, and FFA levels in C57Bl6 and ApoE−/− mice fed a western diet ( Table 4). Treatment of pNaKtide also significantly decreased plasma LDL levels in C57Bl6 and ApoE−/− mice fed a western diet (Table 4). Further, our results showed that both strains of mice fed a western diet had decreased plasma HDL levels (Table 4) and this decrease was reversed by pNaKtide. Generation of ROS has been implicated in the pathogenesis of NASH and atherosclerosis. Our results showed that administration of pNaKtide decreased plasma ROS levels in both strains of mice fed a western diet (Table 4).  The purpose of using the ApoE−/− mouse was to examine the atherosclerosis process. Bright field images of dissected aortas were taken to visualize and quantify lesion size in ApoE−/− mice. In both the whole closed aorta and open aorta images ( Fig. 5A and B respectively), ApoE−/− mice fed a western diet had increased plaque size. This was significantly decreased by pNaKtide treatment. These data were confirmed with Sudan IV staining for lipid deposition (Fig. 6A). The Sudan IV staining was significantly decreased in pNaKtide treated ApoE−/− mice, which demonstrated decreased lipid deposition. Experiments with rhodamine-labeled pNaKtide did not demonstrate pNaKtide localization to aortic plaques ( Supplementary Fig. 1B). Oil Red O staining of the aorta demonstrated increased lipid accumulation in ApoE−/− mice fed a western diet compared to the control group, and treatment with pNaKtide significantly decreased this lipid deposition (Fig. 6B). Furthermore, H&E staining of the aorta revealed a significant increase in cross-sectional lesion area with intimal thickening, acellular matrix of lipid pool, mixed inflammatory cell infiltrate, and necrotic area in ApoE−/− mice fed a western diet (Fig. 6C). All of these outcomes-lesion size, necrotic core area, inflammatory cell infiltration, and intimal thickness improved with pNaKtide treatment (Fig. 6C).

Discussion
This study demonstrates that Na/K-ATPase amplification of oxidant signaling is important in the pathophysiology of NASH and atherosclerosis in the murine models studied. We report that the metabolic syndrome phenotype, present in both C57Bl6 and ApoE−/− mice fed a western diet, improved with pNaKtide treatment which attenuated Na/K-ATPase induced oxidant amplification 20 . Obesity, as measured by body weight and visceral fat weight, was significantly reduced in C57Bl6 mice but not in ApoE−/− mice treated with the pNaKtide. We suggest that this is a consequence of the ApoE−/− mouse being relatively resistant to weight gain with the western diet 21 . In order to determine the mechanism by which pNaKtide affected adiposity, we utilized the CLAMS system to measure metabolic rate. We observed that both energy expenditure and activity level were significantly increased in pNaKtide treatment groups compared to animals fed a western diet, suggesting that increased energy expenditure is at least partly responsible for reduced adiposity in mice fed a western diet. Adipose mitochondria regulate whole-body energy metabolism via dissipating energy and generating heat in adipose tissue 8 . PGC1α and CPT-1 are essential for adipose tissue fatty acid oxidation 8,22,36 . UCP-1 and 2 play important roles in the control of energy expenditure by uncoupling respiration from ATP synthesis, thereby dissipating energy as heat and affecting energy metabolism efficiency 37,38 . In our study, we have shown that C57BL6 and ApoE−/− mice  fed a WD have decreased CPT-1, UCP-1, UCP-2, and PGC1α mRNA expression levels in adipose tissue. This was significantly improved with pNaKtide treatment. Increased CPT-1 and PGC1α expression with pNaKtide may be related to an increase in fatty acid oxidation 8 . Given the established relationship between UCP-1 and 2 and thermogenesis, pNaKtide may increase metabolic rate and energy metabolism in adipose tissue 20 . Overall, we suggest that pNaKtide increases fat utilization by increasing mitochondrial fatty acid oxidation in adipose tissue, oxygen consumption, and metabolic rate leading to an overall decrease in both body weight and visceral adiposity. Since obesity is closely associated with NASH, the effect of pNaKtide on steatohepatitis was evaluated. According to the two-hit hypothesis, hepatic steatosis appears to be a prerequisite for subsequent events that lead to NASH 39 . Obesity and insulin resistance result in increased release of FFAs from adipocytes and increased hydrolysis of TGs, which contribute to elevated plasma levels of FFA 40 . Furthermore, increased FFAs induce oxidative stress via ROS generation 25 , which may initiate the Na/K-ATPase/ROS amplification pathway to propagate steatosis and NASH. Treatment with pNaKtide showed significant attenuation of hepatic steatosis as evident by decreased lipid staining, FAS expression, and TG and FFA concentrations in the livers of C57Bl6 and ApoE−/− mice fed a western diet. Also, pNaKtide attenuated CD36 expression, which we have previously linked to Na/K-ATPase signaling 41 . In addition, ALT, a well-established marker of liver injury, was also decreased by pNaKtide treatment 42 .
Oxidative stress and inflammation are known to underlie the etiopathogenesis of NASH 43,44 and can be categorized as the second hit with regard to the two hit hypothesis. pNaKtide decreased hepatic α1 carbonylation, p-Src, and downstream p-ERK expression to attenuate Na/K-ATPase-induced ROS amplification. Mitochondria play a central role in ATP production and energy expenditure through fatty acid oxidation [31][32][33] . Our results showed that pNaKtide treatment increased hepatic expression of genes involved in fatty acid oxidation including CPT-1, PGC1α and LCAD in the setting of caloric excess, to ameliorate the NASH phenotype. Collectively, it appears that pNaKtide, through its mitigation of ROS, has a favorable effect on mitochondrial biogenesis and fatty acid oxidation in the setting of a WD. It promotes increased substrate utilization, decreased lipid storage, and most importantly minimizes the impact ROS has on these processes, therefore limiting the impact of a second hit.Consequences of oxidative stress (ROS) include lipid peroxidation, which can cause direct damage to hepatocytes and induce an inflammatory response with upregulation of inflammatory cytokines such as MCP-1 and IL-6 45 . We have shown TBARS (a marker of oxidative stress), MCP-1 and IL-6 are all decreased with pNaKtide. Further, our results show that administration of pNaKtide significantly attenuated WD-induced inflammatory cell infiltration in hepatic tissue. This close interaction of ROS and inflammatory cytokines may be how pNaKtide (via the Na/K-ATPase signaling cascade) is able to mitigate the inflammatory component of the second hit, necessary for the development of NASH. With regard to fibrosis, prior studies have shown that the Na/K-ATPase signal cascade, once initiated, activates PKCδ through ROS amplification. PKCδ then phosphorylates Fli-1, which in turn, increases collagen expression [16][17][18][19] . We have similarly shown an increase in hepatic collagen expression in WD fed mice, and pNaKtide significantly decreased collagen deposition. Overall, there was significant attenuation of NASH in C57Bl6 and ApoE−/− mice fed a WD by pNaKtide, as evidenced by decreased lipid accumulation, inflammatory cell infiltration, and trichrome staining for fibrosis. This is supported by findings of decreased markers of lipogenesis (FAS, liver TG/FFAs, CD36), inflammation (IL-6, MCP-1, F4/80), and fibrosis (fibronectin, MMP9, MMP13, collagen-1). We propose that pNaKtide treatment, by decreasing ROS through the Na/K-ATPase pathway, was sufficient to suppress the oxidative stress and inflammation necessary to attenuate steatohepatitis.
NASH is associated with insulin resistance (IR), which results in hypertriglyceridemia and hyperglycemia, which in turn, increases plasma FFAs in the circulation. Increased levels of FFAs in plasma induce oxidative stress via ROS generation 46 . Dyslipidemia is frequently observed in patients with NASH, and treatment of dyslipidemia plays a critical role in the overall management of these patients. pNaKtide improved insulin sensitivity and dyslipidemia, which prompted an examination of how pNaKtide affected vascular disease. Increased levels of circulating FFAs and oxidative stress lead to increased lipid deposition within the vasculature, atherosclerosis, and ultimately cardiovascular complications 46 . Elevated LDL levels have been associated with an increase in the amount of cholesterol entering the plaque 47,48 . More importantly, an increase in serum HDL may contribute to active LDL removal from the vessel wall and from macrophage or foam cells 49 . In the C57Bl6 mouse fed a western diet, fatty streaking was markedly reduced by pNaKtide. We further saw attenuation of aortic atherosclerosis in the ApoE−/− mouse fed a western diet. We suggest that pNaKtide's beneficial effect on atherosclerosis was secondary to a favorable systemic lipid profile. The pNaKtide significantly reduced plasma LDL and TG levels and increased HDL 50 . Whether the plaque decrease observed in this study will translate into significant reductions in clinical events is yet to be determined, however modifying the levels of harmful and protective lipids should still be an important clinical objective. Taken together, this study demonstrates that pNaKtide improves the metabolic syndrome phenotype, specifically obesity, NASH, insulin resistance, dyslipidemia, and atherosclerosis, effects that are mediated by blockage of the Na/K-ATPase/ROS amplification loop. Unfortunately, we were only able to study male animals in the current study. Certainly, the effects of gender and female sex hormones on the development of oxidant stress and obesity may be extremely important.
At this juncture, we would offer a disclaimer that there are a number of interventions that have been shown to be effective in improving the perturbations associated with obesity in these animal models, and some of these have even been found to be effective in clinical practice. However, we would argue that our approach focusing on Na/K-ATPase induced oxidant amplification is novel and potentially presents a new and effective target for therapeutic intervention in the treatment of obesity and its related manifestation dyslipidemia, NASH and atherosclerosis. It should not be forgotten that obesity, metabolic syndrome, diabetes and cardiovascular disease present an increasing burden on healthcare systems and cost in the world today. The approach outlined in this report offers a portal to decreasing the increasing burden that obesity places on society.
In conclusion, we noted that oxidant stress characterized the metabolic syndrome, NASH and vascular abnormalities induced by a western diet in both C57Bl6 and ApoE−/− mice. We further noted that addressing Na/K-ATPase signaling associated oxidant amplification with pNaKtide ameliorated these abnormalities. Should these data be confirmed in humans, strategies like pNaKtide, which focus on this oxidant amplification loop, may potentially augment our clinical approach to these problems.

Material and Methods
Experimental Design. All animal studies were approved by the Marshall University Animal Care and Use Committee in accordance with the National Institutes of Health Guidelines for Care and Use of Laboratory Animals. C57Bl6 mice and ApoE knockout mice (6-8 weeks old, male) were purchased from Jackson Laboratory. Upon arrival to the Byrd Biotechnology Center, ARF, Animal Research Facility, mice were placed in cages and were fed normal chow diet and had access to water ad libitum or were fed Western Diet (WD) and had ad libitum access to high fructose solution. Western diet containing fructose is a well-known model of diet induced metabolic syndrome, and it contributes to chronic metabolic imbalance and to the development of NASH and atherosclerosis [51][52][53] . WD was purchased commercially from Envigo (Indianapolis, IN). WD contained 42% fat, 42.7% carbohydrate, and 15.2% protein yielding 4.5 KJ/g. Fructose was purchased commercially from Alfa Aesar (Ward Hill, MA). Fructose was made at a concentration of 42 g/L, yielding 0.168 KJ/mL. The animals were randomly divided into 4 groups (8-10 mice per group) as follows: (1) Control, (2) Control + pNaKtide, (3) WD, and (4) WD + pNaKtide. The number of animals in each group was determined by power analysis following assumptions derived from our previous study with mice 54 , using a variance of 0.2 within the groups, power of 0.80, and alpha error of 0.05. After 4 weeks of control or WD diet respectively, group 2 and group 4 were injected with pNaKtide for 8 weeks (dissolved in saline and injected I.P. at a dose of 25-mg/kg-body weight every 7 days. The body weight was measured every week. At the end of the 12-week period, mice were placed on an 8-hour fast, anesthetized with sodium pentobarbital (65 mg/kg, I.P.) and blood was obtained from the tail vein for measurement of glucose using a glucometer and measurement of insulin using ELISA assay kit (Abcam, Cambridge, MA). At the time of sacrifice, body weight, visceral fat content, and liver weight of all mice were measured. Liver tissue and aortas were flash frozen in liquid nitrogen and maintained at −80 °C until assayed. Blood samples were collected for lipid profile measurement. Our results showed that there was no significant difference between the Control and Control + pNaKtide C57Bl6 group with regard to body weight ( Supplementary Fig. S2A), glucose tolerance ( Supplementary Fig. S2B), triglycerides ( Supplementary Fig. S2C), HDL (Supplementary Fig. S2D), and LDL ( Supplementary Fig. S2E). Therefore we proceeded without the Control + pNaKtide group in subsequent C57BL6 and ApoE knockout mouse studies.
Indirect calorimetry and locomotor activity. At the end of the 12-week experimental period, energy expenditure and locomotor activity were measured using an eight-chamber CLAM (Columbus Instruments, Columbus, OH, USA). In this system, total oxygen consumption (VO2) and carbon dioxide production (VCO2) were measured, and VO2 was converted to individual heat production (kcal/hour) by Columbus software. This software calculates the heat production by multiplying the calorific value CV = 3.815 + (1.232 × RER) by the observed VO2 (Heat = CV × VO2). The energy expenditure is then calculated as a ratio of heat produced divided by body mass. A system of infrared beams detects movement of animals in CLAMS, and locomotor activity was determined as ambulatory count, the number of times different beams were broken in either the x-or y-axes during an interval. All mice were acclimatized to monitoring cages for 24 hours prior to an additional 48 hours of recordings under the regular 12-hour light-dark cycle.

Blood measurement of LDL, HDL, Triglycerides and Free Fatty Acids (FFA). Plasma LDL and
HDL levels were determined using an ELISA Assay according to manufacturer protocols (Abcam, Cambridge, MA). Triglycerides and FFA levels were quantified using a Quantification Assay Kit according to manufacturer protocols (Abcam, Cambridge, MA).
Blood ROS and hepatic TBARS measurement. Plasma ROS levels were determined using the OxiSelect TM In Vitro ROS Assay Kit according to manufacturer's protocols (Cell Biolabs, Inc, San Diego, CA). Hepatic oxidative injury was measured as TBARS using an assay kit according to manufacturer's protocol (Cayman Chemical, Ann Arbor, MI). Liver samples were homogenized in a buffer solution containing 50 mM tris-HCL (pH 7.4) and 1.15% KCL and then centrifuged. The supernatant was used for the assay. Data were normalized to total protein and presented as micromoles per milligram of protein.
Glucose tolerance test. Glucose clearance was determined using an intraperitoneal glucose tolerance test before termination of the experiment. Mice were fasted for 8 h, after which a glucose solution (2 g/kg body weight, injected as a 10% solution) was injected into the peritoneal cavity. Samples were taken from the tail vein at 0, 30, 60, 90, and 120 min after glucose injection. Blood glucose was measured using the Accutrend Sensor glucometer. Determination of homeostasis model assessment of insulin resistance. The HOMA-IR was calculated from mouse blood using glucose and insulin concentrations obtained after 8 hours of food withdrawal, using the following formula: Distribution of rhodamine B labeled pNaKtide. Mice were injected (by i.p.) without (as control) or with rhodamine B labeled pNaKtide (25 mg/Kg body weight). Three hours after injection, the mice were sacrificed and the hepatic tissues were imaged and analyzed. The images were taken at laser power 5% (emission readings for rhodamine B are 580-650 nm) with a Leica SP5 TCS II equipped with coherent chameleon multiphoton vision II (IR) laser and analyzed by Leica LAS/AF software.
Determination of Triglyceride and FFA levels in hepatic tissue. For triglyceride measurement, liver samples were homogenized in ice-cold phosphate-buffered saline (PBS). Tissue lipids were extracted with methanol/chloroform (1:2), dried, and resuspended in 5% fat-free bovine serum albumin. Triglyceride levels were determined using a commercially available kit according to the manufacture's protocol (Abcam, Cambridge, MA). For FFA measurement, liver tissue was homogenized in 1% (w/v) Triton X-100 in chloroform solution. After centrifugation of samples, the lower organic phase was collected and dried to remove chloroform. The dried lipids were dissolved in fatty acid assay buffer and FFA levels were determined using a commercially available kit according to the manufacturer's protocol (Sigma-Aldrich, St. Louis, MO).
Histopathological examination in hepatic tissue. Liver samples from each group were fixed in 4% paraformaldehyde, dehydrated, embedded in paraffin, and sectioned. Formalin-fixed, paraffin-embedded sections were cut (6 μm thick) and mounted on glass slides. The sections were deparaffinized in xylene and hematoxylin and eosin and Masson's trichrome staining were performed for histological analysis.
Oil Red-O staining. For Oil Red O staining, liver and aorta tissues, which were frozen in OCT compounds, were cut into 6 μm sections, mounted on slides and allowed to dry for 1-2 hours. The sections were fixed with 4% paraformaldehyde (PFA) for 1 hour and then the slides were rinsed with PBS (pH 7.4). After air-drying, the slides were stained in 0.3% Oil Red O solution for 3 minutes. The slides were rinsed with distilled water 2 times and mounted with 87% glycerol. The microphotographs were taken on a Nikon Eclipse 80i microscope equipped with a Nikon camera head DS-Fi1 (Nikon, Japan). For quantitative analysis, the total area of red pixels on the Oil-Red-O stained tissue section was measured by using the Image J software provided by NIH. The data were expressed as the mean ± SEM of percentage of the Oil-Red-O stained areas with respect to total area. Aorta Dissection and Sudan IV staining. Aorta Harvesting. The aorta was dissected and harvested under a stereomicroscope from the iliac bifurcation to the aortic root, including the brachiocephalic trunk, left common carotid artery, and left subclavian artery. The adventitial fat was removed. The aortic trunk was washed with cold PBS and pinned onto a black wax surface.
Whole Aorta Imaging. Bright field images of the dissected aorta were taken with a Leica stereomicroscope (Leica MZ10F; Leica Microsystems, Buffalo Grove, IL) attached to a QImaging Camera (Q26644; Surrey, Canada) at a total magnification of 8x (objective lens was 0.8x and eye piece lens was 10x).
Open Aorta Imaging. Whole aortas were opened longitudinally from the aortic root to the iliac bifurcation and pinned to a black wax surface. Bright field mages were acquired using a Leica stereomicroscope attached to a QImaging Camera at a total magnification of 8x.
Sudan IV Staining. To identify lipid rich intraluminal lesions, the aortas were stained with commercially available Sudan IV (Sigma, St Louis, MO). A 0.5% Sudan IV solution was made using acetone and ethanol at an equal ratio. Tissues were treated with 70% ethanol for 5 minutes followed by Sudan IV for 15 minutes. They were then washed with 80% ethanol for 3 minutes and rinsed with PBS for 3 minutes. Finally tissues were treated with 0.4% PFA for storage and imaging.
Haematoxylin and Eosin Staining. The aorta, stored in OCT, was cut into 6 μm sections and stained with haematoxylin and eosin for histological analysis.
Quantification of Aortic Lesions. Quantification of atherosclerotic lesions was done using Image J 1.49 V (NIH). The amount of lesion formation in each animal was expressed as a ratio of plaque integral density to total surface area of the aorta.
Measurement of c-Src and ERK1/2 phosphorylation. Whole cell lysates from hepatic tissue were prepared with NP-40 buffer and activation of c-Src and ERK 1/2 was determined as previously described by Yan et al. 15,55 . After immunoblotting for phospho-c-Src and phospho-ERK1/2, the same membrane was stripped and immunoblotted for total c-Src and total ERK 1/2. Activation of c-Src and ERK1/2 was expressed as the ratios of phospho-c-Src/ total Src and phospho-ERK1/2/total ERK 1/2, respectively with both measurements normalized to 1.0 for the control samples.
Assessment of protein carbonylation. Whole-cell lysates from hepatic tissues were prepared with NP-40 buffer and western blotting for protein carbonylation assay was done 55 . The signal density values of control samples were normalized to 1.0 with Ponceau S staining as a loading control. Western blot analysis. Liver was pulverized with liquid nitrogen and placed in a homogenization buffer. Homogenates were centrifuged, the supernatant was isolated, and immunoblotting was performed. The supernatant was used for the determination of Collagen-1 and PGC1α as previously reported 36,56 . Loading conditions were controlled for using tubulin (collagen1) and actin (PGC1α). Mitochondrial extraction was performed on hepatic tissue by using a mitochondrial isolation kit (Abcam, Cambridge, MA). In brief, liver tissues were minced, and placed in pre-chilled dounce homogenizer. The homogenate was centrifuged at 1000 g for 10 mins at 4 degrees and the supernatant was saved. The supernatant was spun at 12000 g for 15 mins at 4 degrees and the pellet was saved. The pellet was washed and resuspended in isolation buffer and protease inhibitor, centrifuged at 12000 g for 15 mins. The pellet was again collected and the process was repeated. The pellet was resuspended in isolation buffer and protease inhibitor and used immediately. This mitochondrial homogenate was used for the determination of CPT-1 and LCAD and Porin was used as a loading control.
RNA extraction and real-time PCR. Total RNA was extracted from liver and adipose tissue using RNeasy Protect Mini kit (QIAGEN, Maryland, USA) according to manufacturer's instructions. Total RNA (1 μg) was transcribed into cDNA using GeneAmp kit (Applied Biosystems, Branchburg, NJ, USA) reverse transcription reagents. Total RNA was analyzed by a quantitative real time polymerase chain reaction 57 . Real-time PCR was performed using SYBR Green PCR Master Mix (Applied Biosystems) on a 7500 HT Fast Real-Time PCR System (Applied Biosystems). Specific primers used were FAS, CD36, IL-6, F4/80, MCP-1, MMP9, MMP13, fibronectin, UCP-1, UCP-2, CPT-1, LCAD, PGC1α and GADPH. Each reaction was performed in triplicate. The comparative threshold cycle (Ct) method was used to calculate the fold amplification as specified by the manufacturer. All experimental samples were normalized using actin as an internal control and normalization was performed in separate reactions.
Statistical analyses. Data were tested for normality and then subjected to parametric analysis. When more than two groups were compared, one-way ANOVA was performed prior to comparison of individual groups, and the post-hoc t-tests were adjusted for multiple comparisons using the Tukey-Kramer correction. Data are presented as mean ± SEM.