Animals and experimental design

All experimental protocols involving animals conformed to the procedures described in the Guiding Principles for the Use of Laboratory Animals. The study was approved by the Animal Committee of Federal University of São Paulo, UNIFESP, SP, Brazil.

Male Wistar rats (8 weeks old), weighing approximately 250 g, were obtained from the Centro de Desenvolvimento de Modelos Experimentais, Federal University of São Paulo, SP, Brazil. They were maintained under controlled conditions of temperature (24 ± 2°C), 12 h light–12 h dark cycles and with free access to water and commercial diet (Nuvital, Paraná, Brazil). All animals were acclimatised for 7 d before the experiment, fed ad libitum standard pellet chow and fresh water.

A total of eighteen rats were randomly divided into three groups (six animals per group). To induce a hypercholesterolaemic state, twelve animals were treated with a standard rat chow diet added with 1 % (w/w) cholesterol (C8503; Sigma Chemical Company, St Louis, MO, USA) and 0·25 % (w/w) cholic acid (C1254; Sigma Chemical Company; cholesterol-enriched diet), according to the methodology described by Manzoni et al. ⁽Reference Manzoni, Rossi and Carlos²⁰⁾. Immediately after weaning, animals were fed a cholesterol-enriched diet for 5 weeks to induce hypercholesterolaemia. Animals were divided into two groups: six animals without any treatment (positive control) and six animals receiving grape juice concentrate, freshly prepared, dissolved in their drinking-water in the final week only (in the final 7 d). A total of six animals served as the negative control group. Body weight was recorded weekly.

At the end of the experimental period, the rats were killed with 0·4 % sodium pentobarbital (1 ml/kg, intraperitoneally). The livers were longitudinally bisected for morphological and biochemical examinations. For this purpose, a fragment from the liver was homogenised in two volumes of NaCl at 0·9 % to promote cell separation. Then, a volume of 20 μl supernatant was subjected to a single-cell gel (comet) assay⁽Reference Andersen, Ribeiro and Alvarenga²¹⁾. The remainder of the tissues were fixed in 10 % buffered formalin (Merck, Darmstadt, Germany), embedded in paraffin blocks and stained with haematoxylin and eosin (Merck, Whitehouse Station, NJ, USA).

Grape juice concentrate intake

Animals were given 222 mg/d of grape juice concentrate (G8000™; Golden Sucos, Farroupilha-RS, Brazil) in their drinking-water. The amount of polyphenols was calculated to be equivalent to four glasses (200 ml each) of natural grape juice⁽Reference Gollucke, Souza and Tavares²²⁾ and adjusted to the fastest animal metabolism (twice as fast as humans). According to the American Dietetic Association, human consumption of approximately 200–500 ml of grape juice presents moderate to strong evidence of positive physiological effects⁽²³⁾.

Determination of total phenols and in vitro antioxidant activity of grape juice concentrate

Total phenols were measured by the Folin–Ciocalteu assay⁽Reference Singleton and Rossi²⁴⁾, using gallic acid (Sigma-Aldrich, St Louis, MO, USA) for the standard curve, and the results were expressed as mg gallic acid equivalents/kg. The readings (in triplicate) were taken at 740 nm, using a Genesis 2 spectrometer. For the evaluation of in vitro antioxidant activity, the 1,1-diphenyl-2-picrylhydrazil (Sigma-Aldrich, Steinheim, Germany) assay was used based on the methods of Brand-Williams et al. ⁽Reference Brand-Williams, Cuvelier and Berset²⁵⁾, as modified by Kim et al. ⁽Reference Kim, Lee and Lee²⁶⁾. Absorbance was measured with a Beckman spectrometer at 517 nm before the addition of samples and after 30 min. The difference was plotted on a vitamin C (ascorbic acid) (Merck, USA) standard curve. Analyses were carried out in triplicate and the results were expressed in mg vitamin C equivalents/kg.

Characterisation of grape juice concentrate by electrospray ionisation-mass spectrometer fingerprinting

ESI-MS data were collected in the negative-ion mode on an API5000 mass spectrometer (Applied Biosystems/MDS Analytical Technologies, ON, Canada). Typical ESI-MS conditions were as follows: curtain gas, ion source gas and ion transfer voltage were 10 V, 15 and 4 kV, respectively, with a desolvation temperature of 200°C. To each sample (0·1 ml), 1 ml of a methanol–water solution (7:3, v/v) and 0·1 ml of a methanol solution of ammonia (0·1 %, v/v) were added. The diluted solution was then directly infused into the ESI source at a flow rate of 10 μl/min via a microsyringe pump. The mass analyser was set to scan along a m/z range of 50–1000. ESI-MS/MS experiments were carried out by selection of a specific ion by Q1 and then submitting this to collision-induced dissociation with Ar in a collision chamber. The collision energy was optimised for each component, varying from 15 to 50 V. ESI-MS data from the sample were extracted using the Analyst 1.4.1 (Applied Biosystems/MDS Analytical Technologies). Mass spectrum data were accumulated over 60 s. The degree of confidence for this method is 99 %.

Measurement of cholesterol levels

Measurements of total cholesterol were performed through specific enzymatic kits as follows: to determine total cholesterol, the fast colour method was employed with reagents from the Sera Pak-Ames-Analyzer (RAXT-Technicon, Ames, IA, USA).

Histopathological analysis

Histopathological changes, including steatosis and inflammation, were analysed by the semi-quantitative method (Table 1) according to Zhang et al. ⁽Reference Zhang, Xu and Liu²⁷⁾.

Table 1 Score criteria for hepatopathological changes (including steatosis and inflammation)⁽Reference Kim, Lee and Lee²⁶⁾

PMN, polymorphonuclear leucocyte.

Single-cell gel (comet) assay and challenge assay

The peripheral blood and liver samples collected from each animal were divided into two aliquots of 30 μl each to study (1) basal DNA damage and (2) DNA damage due to oxidative stress as described elsewhere⁽Reference Andersen, Ribeiro and Alvarenga^21, Reference Saran, Tiwari and Reddy²⁸⁾. For this purpose, the first aliquot was immediately processed for the comet assay to assess basal DNA damage. The second aliquot was treated with a known oxidative DNA damage, H₂O₂ (Sigma-Aldrich). On the basis of previous experiments carried out in our laboratory, samples were treated with 10 μm-PBS (at 4°C for 5 min). Samples were then washed three times with PBS to remove any residual mutagen and processed for the comet assay.

The protocol used for the single-cell gel (comet) assay followed the guidelines proposed by Tice et al. ⁽Reference Tice, Agurell and Anderson²⁹⁾. Briefly, a volume of 10 μl peripheral blood or cellular suspensions from the liver (approximately 1 × 10⁴ cells) were added to 120 μl of 0·5 % low-melting-point agarose at 37°C, layered onto a pre-coated slide with 1·5 % regular agarose and covered with a coverslip. After brief agarose solidification in a refrigerator, the coverslip was removed and the slides were immersed in lysis solution (2·5 m-NaCl, 100 mm-EDTA – Merck, Darmstadt, Germany; 10 mm-Tris–HCl buffer, pH 10 – Sigma Aldrich; 1 % sodium sarcosinate – Sigma; with 1 % Triton X-100 – Sigma; 10 % dimethyl sulphoxide – Merck) for approximately 1 h. Before electrophoresis, the slides were left in alkaline buffer (0·3 mm-NaOH (Merck) and 1 mm-EDTA (Merck); pH>13) for 20 min and electrophoresed for another 20 min at 25 V (0·86 V/cm) and 300 mA. After electrophoresis, the slides were neutralised in 0·4 m-Tris–HCl (pH 7·5), fixed in absolute ethanol and stored at room temperature until analysis. In order to minimise extraneous DNA damage from ambient UV radiation, all steps were performed with reduced illumination.

A total of fifty randomly captured comets from each slide⁽Reference Hartmann, Agurell and Beevers³⁰⁾ were blindly examined at 400 × magnification, using a fluorescence microscope (Olympus, Orangeburg, NY, USA) connected through a black and white camera to an image analysis system (Comet Assay II; Perceptive Instruments, Haverhill, Suffolk, UK). This computerised image analysis system records images, computes the integrated intensity profiles for each cell, estimates the comet cell components and then evaluates the range of derived parameters. Undamaged cells have an intact nucleus without a tail and damaged cells have the appearance of a comet. To quantify the DNA damage, the tail moment was evaluated. The tail moment was calculated as the product of the tail length and the fraction of DNA in the comet tail. The comet tail moment is positively correlated with the level of DNA breakage in a cell. The mean value of the tail moment in a particular sample was taken as an index of DNA damage in such a sample.

Immunohistochemistry

Liver sections of 3 μm were deparaffinised in three changes of xylene and rehydrated in a graded series of ethanol to distilled water. For antigen retrieval, slides were placed in 0·01 m-citrate-buffer (pH 6·0) and heated in a steamer for 30 min. Endogenous peroxidases were quenched by incubating in 3 % H₂O₂ for 20 min at room temperature. The sections were incubated overnight at 4°C with a primary antibody: COX-2 mouse polyclonal antibody (1:400; Santa Cruz Biotechnology, Santa Cruz, CA, USA). Subsequently, the sections were incubated with a biotinylated secondary antibody (LSAB, Dakocytomation, Denmark) for 30 min, washed in PBS and incubated with a streptavidin–peroxidase conjugate (LSAB) for 30 min. Finally, the reaction was developed using 3,3′-diaminobenzidine tetrahydrochloride (Sigma) for 5 min. The slides were briefly counterstained in haematoxylin and dehydrated, and coverslips were added. Negative and positive controls were run simultaneously. Positive controls were represented by mammary tissue. Negative controls were made by eliminating the primary antibody.

Immunostaining was scored by two trained independent observers (B. B. de M. and D. A. R.) without prior knowledge of the histopathological parameters. Discordant cases were reviewed and agreed upon before the data had been statistically analysed. For this purpose, immunohistochemically stained liver sections were analysed for the percentages of immunopositive cells in areas diagnosed as normal and in damaged liver cells. A total of 1000 liver cells were evaluated in three to five fields at 400 ×  magnification. All values were used as labelling indices. Such a protocol was established in previous studies conducted by our research group⁽Reference Fracalossi, Miranda and Oshima³¹⁾.

Statistical methods

Initial body weight, weight gain, total cholesterol and comet assay data were analysed by one-way ANOVA followed by Tukey's test. Statistical analyses for immunohistochemistry data and histopathological scores were assessed by the Kruskal–Wallis non-parametric test, followed by post hoc analysis (Dunn's test), using the SPSS software package (version 1.0; SPSS Institute, Chicago, IL, USA). A P value < 0·05 was considered statistically significant.