Ethical statement

All procedures were approved by the Ethics Committee on Animal Care of the Health Sciences Center, Federal University of Rio de Janeiro (protocol no. IBCCF 140/13), which follows the principles adopted in the UK and Brazil according to Brazilian Law no. 11.794/2008⁽Reference Drummond^26, Reference Marques, Morales and Petroianu²⁷⁾.

Experimental animals and procedures

Wistar rats were obtained from the Center of Reproduction Biology of the Federal University of Rio de Janeiro, Rio de Janeiro, Brazil. They were acclimated and maintained in individual cages with free access to water and food in a room with controlled temperature (23 ± 2°C) and 12 h light–12 h darkness cycles (lights on from 07.00 to 19.00 hours). Wistar rats are experimental models frequently used in evaluation of the consequences of metabolic programming^{(Reference Franco, Fernandes and Rocha7,Reference Oliveira, Souza and Souza8,Reference Ramaiyan, Bettadahalli and Talahalli17,Reference Wyrwoll, Mark and Mori19,Reference Hou, Ji and Wang20,Reference Zheng, Xiao and Zhang28)} , because rodents have short gestation and lactation periods, allowing the rapid evaluation of transgenerational transmission⁽Reference Armitage, Khan and Taylor²⁹⁾. Besides that, genetic and environmental influences can be carefully controlled in these experimental models. The relevance of our study is that this experimental model simulates the increased consumption of HFD and obesity rates among women in reproductive age⁽Reference Vahratian³⁰⁾, and its correlation with metabolic obesity among adolescent offspring reported by epidemiological observations⁽Reference Oken, Rifas-Shiman and Field³¹⁾. Then, our model allows to investigate the perinatal insult impact on phenotype and molecular changes of offspring⁽Reference Armitage, Khan and Taylor²⁹⁾, inferring the molecular mechanism involved in the human observations.

Twenty-six female Wistar rats, 60 d old and weighing 190–220 g, were randomly distributed in two experimental groups: standard diet (STD) or HFD (thirteen per group). The STD group received an STD for rodents (9 % of the energy as fat), and HFD group received an HFD (28⋅6 % of the energy as fat – lard was used as the major fat source) for 8 weeks before mating and during pregnancy and lactation⁽Reference Franco, Fernandes and Rocha⁷⁾. During mating, two female rats of the same group were housed with one male rat (150 d old). After this, female rats were housed in individual cages during pregnancy and lactation to avoid stressful environment. The maternal comportment was evaluated, and the maternal stress was discarded by absence of killed puppies by dams. At birth, litters were adjusted to six males for each dam aiming to improve lactation performance⁽Reference Fischbeck and Rasmussen³²⁾. STD and HFD offspring received STD (the same perinatal STD) during the postnatal period, from weaning (21 d old) until adulthood (150 d old).

Our HFD is moderately high-fat compared with most experimental models that generally use diets with 50 % of the energy as fat⁽Reference Zheng, Xiao and Zhang^28, Reference Yokomizo, Inoguchi and Sonoda³³⁾. The HFD was manually produced in our laboratory using the ingredients described at Table 1, including the commercial STD chow. Diet composition followed the American Institute of Nutrition recommendations (AIN-93) for micronutrients⁽Reference Reeves, Nielsen and Fahey³⁴⁾ and was described before⁽Reference Franco, Fernandes and Rocha^7–Reference Franco, Dias-Rocha and Fernandes⁹⁾. Both diets contained approximately 16⋅3 kJ/g of energy (isoenergetic) and their macronutrients compositions are described at Table 2. The HFD was composed by a moderate increased lipid content with protein and carbohydrate contents within the range recommended for rodents (AIN-93), which avoided the negative impact of low-protein or low-carbohydrate diets⁽Reference de Oliveira, Gomes and Miranda^35, Reference Koski and Fergusson³⁶⁾. The differences between macronutrient compositions of diets were not tested statistically, because we estimated the diet composition by ingredients composition described at ingredient label. The fatty-acid compositions of diets were analysed by gas chromatography. The HFD showed higher SFA content than STD (P < 0⋅01), and its detailed fatty-acid composition is described at Table 3.

Table 1. Diet composition (g/kg) on the basis of the American Institute of Nutrition (AIN)-93G diet formulation

HFD, high-fat diet; BHT, butylated hydroxytoluene.

Table 2. Diet macronutrient composition

* To convert kcal to kJ, multiply by 4·184.

Table 3. Fatty acid composition of the experimental diets (µg/mg of chow)

STD, standard diet; HFD, high-fat diet; N.D., not detected.

* Fatty acids were quantified by GC/MS determining peak-area ratios with the 9 : 0 and 19 : 0 internal standards. We used three samples per group.

In the adolescence period⁽Reference Schneider³⁷⁾, two male rats of each litter were randomly allocated at soyabean oil (SO) or FO group in individual cages. The remaining pups were used in another experimental design⁽Reference Oliveira, Souza and Souza⁸⁾. Then, the experimental design had four experimental groups: STD or HFD offspring that received SO (source of n-6 PUFA; Liza®, Cargill) (n 12 and 9, respectively) and STD or HFD offspring that received FO (source of n-3 PUFA; Fagron) (n 12 and 9, respectively). Oil administration was given daily by gavage (4 ml/kg body weight) from 25 to 45 d old. Each capsule of FO had 95⋅5 mg/ml of EPA and 61 mg/ml of DHA, resulting in a dose of 0⋅244 g/kg of DHA and 0⋅380 g/kg per d. This DHA dose adjusted to human⁽Reference Reagan-Shaw, Nihal and Ahmad³⁸⁾ is in a dose range used in human experimental design with FO supplementation during the adolescence period⁽Reference McNamara, Strimpfel and Jandacek^39–Reference de Ferranti, Milliren and Denhoff⁴¹⁾. SO was used as control to exclude lipid load effect, ensuring that the results are derived from the different types of fatty acids used in the treatment. Furthermore, SO is a lipid source recommended for rodents according to the AIN-93⁽Reference Reeves, Nielsen and Fahey³⁴⁾, and represents the main fatty acid present in the Western diet (n-6 PUFA)⁽Reference Spector⁴²⁾.

We performed an oral glucose tolerance test with the animals at 147 d of age. After 12-h fasting, capillary blood glucose was measured from a tail incision, followed by oral glucose (d- (+) -glucose; VETEC) administration (2 mg/g of body weight). Glycaemia was also measured at 15, 30, 60 and 90 min after glucose administration (One Touch Ultra Mini device; Johnson and Johnson).

During the experiment, we did not observe adverse events or features of stressed animals, such as aggressive behaviour, hair loss or body weight loss. At 150 d of age, rats were killed by decapitation. Serum was obtained from trunk blood (after centrifugation at 1000 g, 4°C, 20 min) and kept frozen at −20°C for measurements of hormone levels and biochemical parameters. Representative depots of visceral white adipose tissue (retroperitoneal and epididymal) were dissected, weighed and returned to eviscerated carcass, to evaluate the adiposity. Liver was harvested, snap frozen in liquid nitrogen and stored at −70°C prior to extraction of total lipid, protein and RNA.

Fatty-acid composition of the experimental diets

The GC/MS assay was used to investigate the fatty-acid profile in experimental diets (STD and HFD). The lipid sample was dissolved in a toluene and 1 % sulfuric acid in methanol solution. GC/MS analysis was carried out on a Shimadzu GCMS-QP2010 Plus system, using an HP Ultra 2 (5 % phenyl-methylpolysiloxane), Agilent (25 m ×0⋅20 mm × 0⋅33 μm). Injector was set at 250°C. Column temperature was programmed from 40 to 160°C at 30°C/min, 160 to 233°C at 1°C/min, 233 to 300°C at 30°C/m and held at 300°C for 10 min. Electro ionisation (EI-70 eV) and a quadrupole mass analyser operated in scans from 40 to 440 atomic mass units. Interface was set at 240°C and the ion source at 240°C. The components were identified by comparing their mass spectra with those of the library NIST05 contained in the computer’s mass spectrometer. Retention indices were also used to confirm the identity of the peaks in the chromatogram by Supelco 37 Component FAME Mix (Sigma-Aldrich). Fatty acids were quantified by determining peak-area ratios with the 9 : 0 and 19 : 0 internal standards. We used three samples per group.

Body composition analysis

Total body lipid quantification was performed as previously described⁽Reference Stansbie, Brownsey and Crettaz^43, Reference Souza, Nunes and Paula⁴⁴⁾. Briefly, eviscerated carcasses were weighed, autoclaved and homogenised in distilled water (1:1). Homogenate (3 g) was hydrolysed in a shaking water bath at 70°C for 2 h with 30 % KOH and ethanol, followed by three successive washes with petroleum ether (Vetec) to extract lipids. The petroleum ether phases containing the lipids were dried at room temperature until constant weight was obtained.

Serum lipid profile

Serum total cholesterol (no. 12505), HDL-cholesterol (no. 12557) and TAG (no. 12528) quantification was performed using commercial kits from Biosystems and an automated A15 spectrophotometer (Biosystems S.A.). The serum VLDL-cholesterol and LDL-cholesterol were estimated according to the Friedewald assumption⁽Reference Friedewald, Levy and Fredrickson⁴⁵⁾: VLDL = TAG/5 and LDL = total cholesterol − HDL − TAG/5.

Hormone assays

Serum leptin was measured using specific commercial radioimmunoassay (RIA) kit from Linco Research (no. XL-85K). Total serum thyroxine and total serum triiodothyronine were determined using specific commercial RIA kits from MP Biomedicals (no. 06B-254011 and no. 06B-254215). Serum thyroid-stimulating hormone (TSH) was measured by a specific rat TSH RIA using reagents acquired from the National Hormone and Pituitary Program, as previously detailed⁽Reference Ortiga-Carvalho and Curty⁴⁶⁾. Serum adiponectin was measured by a specific rat Adiponectin ELISA Kit from Merck Millipore (no. EZRADP-62K). All samples were evaluated in duplicate within the same assay according to the manufacturer’s instructions.

Real-time PCR analysis

Real-time PCR assay was used to evaluate the relative mRNA expression of genes encoding PPARα (Ppara), hepatic lipase (Lipc), carnitine palmitoyl transferase-1a (CPT-1a: Cpt1a), leptin (Lep), PPARγ (Pparg), IL-1β (Il1b), IL-6 (Il6), IL-10 (Il10) and TNF-α (Tnf).

Total RNA was isolated from retroperitoneal adipose tissue samples using a commercial RNeasy lipid tissue mini kit (Qiagen), and from liver samples using a commercial SV Total RNA Isolation System (Promega). Total RNA was reverse transcribed using 1 μg of total RNA and a High-Capacity cDNA Reverse Transcription Kit (Applied Biosystems). Products were amplified on Eppendorf MasterCycler RealPlex (Eppendorf) using Maxima SYBR Green qPCR Master Mix (Thermo Scientific). Cycle parameters were 50°C for 2 min and 95°C for 10 min, followed by forty cycles at 95°C for 15 s, 60°C for 30 s, and 72°C for 45 s. The intron spanning primers sequence used in the present study are described in Table 4. Primers were synthesised and tested by Integrated DNA Technologies. Samples and negative controls were evaluated in duplicate in the same assay. Efficiency of each PCR reaction was calculated using a serial cDNA dilution standard curve, and varied from 96 to 100 %. Product purity was confirmed by a single peak in the melting curve analysis. Relative mRNA levels were calculated using standard curve method and normalised by mRNA levels of the reference genes Polr2a (liver) or Rplp0 mRNA (adipose tissue). Results are expressed relative to values of control group (STD offspring that received SO during the adolescence period).

Table 4. Primer sequences for gene expression evaluation

Western blotting analysis

We used the Western blotting assay to evaluate the hepatic content of fatty acid synthase (FAS), CPT-1a, and signal transducer and activator of transcription 3 (STAT3 and pSTAT3). The content of cyclophilin (Cyclo) or glyceraldehyde-3-phosphate dehydrogenase (GAPDH) was used as loading control. Liver samples were homogenised in lyses buffer pH 6⋅4 (50-mm HEPES, 1-mm MgCl₂, 10-nm EDTA, and 1 % Triton X) with protease inhibitor cocktail complete (Roche Diagnostics). After centrifugation of the homogenates, the total protein content of the supernatant was quantified using the Pierce^TM BCA Protein assay kit (Thermo Scientific). Total protein was separated by SDS–PAGE and transferred onto a polyvinylidene difluoride membrane (Hybond-P 0⋅45 µm PVDF; Amersham Biosciences). Membrane was blocked with 5 % non-fat dry milk (Molico, Nestlé) or 5 % bovine serum albumin (INLAB) according to the protein of interest for 1 h at room temperature. Then, membrane was incubated overnight at 4°C with primary antibodies: anti-FAS (Cell Signaling; 1:1000 dilution), anti-CPT-1a (Abcam; 1:3000 dilution), anti-STAT3 (Santa Cruz; 1:400), anti-pSTAT (Santa Cruz; 1:1600) and loading control anti-Cyclo (Thermo Scientific; 1:40 000 dilution) or anti-GAPDH (Cell Signaling; 1:3000 dilution). Membranes were washed and incubated with peroxidase-labelled anti-rabbit IgG antibody (Amersham Biosciences, BKM, England; 1:10 000 dilution) or anti-mouse IgG antibody (Cell Signaling; 1:10 000) for 3 h at room temperature. All blots were then washed and incubated with a luminogen detection reagent (Amersham ECL Prime Western Blotting Detection reagent; Amersham Biosciences or SuperSignal® West Femto Maximum Sensitivity Substrate; Thermo Scientific). Chemiluminescent signal was detect by ImageQuant LAS 4000 equipment followed by densitometric analyses (GE Healthcare Life Sciences).

TLC

Liver total lipids were extracted by the method of Bligh &Dyer⁽Reference Bligh and Dyer⁴⁷⁾ with modifications. After incubation in chloroform–methanol–water solution (2:1:0⋅4, by vol.), samples were centrifuged (1500 g for 20 min at 4°C). Then, the chloroform was added to the supernatant. After centrifugation (1500 g for 20 min) the organic phase was removed and dried in nitrogen. The extracted lipids were analysed by TLC for neutral lipids, using a DC Silicagel 60 plate (Merck Millipore) and standards lipids. The plates were submerged for 10 s in Charring solution (3 % CuSO₄ and 8 % H₃PO₄ (v/v)), then they were dried and heated to 110°C for 5–10 min. TLC plates were analysed by densitometry (GE Healthcare Life Sciences), defining hepatic free cholesterol, NEFA and TAG content.

Statistical analysis

The sample size was calculated by using the G*Power 3.1.9.2 program⁽Reference Faul, Erdfelder and Lang⁴⁸⁾, based in our previous observations of maternal HFD effect on plasma and molecular parameters of the adult offspring⁽Reference Franco, Dias-Rocha and Fernandes⁹⁾ and our previous observations of FO intake effect on plasma and molecular parameters in adolescents rats⁽Reference Oliveira, Souza and Souza⁸⁾. Regarding plasma parameters, a sample size of nine animals per group would provide the appropriate power (1 − β = 0·8) to identify significant differences (α = 0·05) in the variables analysed, using a two-tailed test. For molecular parameters, a sample size of six animals per group would provide the appropriate power (1 − β = 0·8) to identify significant differences (α = 0·05) in the variables analysed, using a two-tailed test. The statistical comparisons were performed using the software GraphPad Prism (GraphPad Software Inc.) showing results as means with their standard errors. Two-way ANOVA were used considering two variables (maternal diet and oil intervention) and significant differences at P < 0⋅05. Tukey’s post-test was used to evaluate differences between columns in only each maternal condition. In each analysis of post-test, we corrected the result for multiple comparisons using statistical hypothesis testing and reported multiplicity adjusted P value for each comparison, using a confidence level of 0⋅05. To data correlation analysis, normality was assessed by the Kolmogorov–Smirnov test, followed by non-parametric Spearman’s correlation test.