Reagents

Laboratory chemicals, namely 5-aminosalicylic acid, 2,4,6-trinitrobenzenesulfonic acid solution (TNBS), 5,5′-dithiobis(2-nitrobenzoic acid) (DTNB), glutathione reductase, L-glutathione reduced (GSH) and oxidized (GSSG) forms, β-NADPH, 5-sulfosalicylic acid, 2-vinylpyridine, 2,3-diaminonaphthalene (DAN), o-dianisidine dihydrochloride, hexadecyltrimethylammonium bromide (CTAB), protease inhibitor cocktail and general laboratory chemicals were purchased from Sigma-Aldrich (St Louis, Missouri, USA). Microcon-10kDa centrifugal filters were obtained from Merck Millipore (Merck KGaA, Darmstadt, Germany).

Rabbit polyclonal antibody to iNOS was purchased from Cell Signalling Technology (Leiden, The Netherlands); rabbit polyclonal antibody to COX-2 was purchased from Abcam (Cambridge, UK); goat polyclonal antibody to MPO was purchased from Santa Cruz Biotechnology (Santa Cruz, CA, USA); mouse monoclonal antibody to β-actin was purchased from Sigma-Aldrich (St Louis, Missouri, USA); anti-rabbit, anti-mouse and anti-goat IgG secondary antibodies were purchased from Abcam (Cambridge, UK).

Blueberry samples

The blueberries (Vaccinium corymbosum L, cultivar Bluecrop) were collected at the time of peak production, from the central region of Portugal. They were obtained from biological agriculture (Biogrêsso, Portugal) and kept frozen at -80°C until use.

Preparation of anthocyanin-rich fraction

The anthocyanin-rich fraction was prepared according to Oszmianski, et al [21], as modified by Youdim (2002) [22]. Briefly, a total extract was obtained by homogenization of 30 g of the frozen fruits in 150 ml of methanol, acetone, water and formic acid mixture (40:40:20:0.1 v/v/v/v). Then, the extract was centrifuged at 2000g for 10 min and the supernatant was dried by rotatory evaporation at 40°C under vacuum. The resulting residue was dissolved in deionized water and applied to an activated Sep-Pak C18 column (Waters Corporation, Milford, Massachusetts, USA). The column was then washed with 2 volumes of acidified water (0.01% HCl) to remove sugars and phenolic acids, and 2 volumes of ethyl acetate to elute other phenolic compounds. The anthocyanins were eluted only in the presence of acidified methanol (0.01% HCl) [23]. This fraction was then dried at low pressure, and further resolubilized in a 0.9% NaCl solution. The anthocyanin-rich extract was kept at -80°C, under nitrogen, until use and will be further referred here as ARF.

Total phenols and total anthocyanins assays

The total content in phenolic compounds was assessed spectrophotometrically by the Folin-Ciocalteau reagent, as described by George et al [24]. Results were expressed as grams of gallic acid equivalents (GAE) per volume of ARF (L) and as milligrams of GAE per 100 g of blueberries.

Total monomeric anthocyanins in the ARF were estimated by a pH differential method described by Giusti et al [25], by using two buffer systems. The fraction was previously diluted at a ratio of 1:800 (v:v) either with 0.025 M KCl (pH 1) or with 0.4 M sodium acetate buffer (pH 4.5) and after an equilibration period (15 min), the absorbance spectrum of each solution was recorded between 400 and 700 nm in a Perkin Elmer Lambda 45 spectrophotometer. The anthocyanin content was calculated in terms of malvidin-3-glucoside (malv3glc) equivalent, using the maximum of absorbance measured around 530 nm, the molar absorptivity of 20200 and the molecular weight of 493.4. The results were expressed as grams of malv3glc equivalents/L of ARF and as milligrams of malv3glc equivalents/100 g blueberries.

HPLC-DAD

The extract was analysed by HPLC with direct injection of the samples (20 μL) (Hitachi L-2130) in a reverse phase C18 column with 250 x 4.6 mm i.d. (Merck KGaA, Darmstadt, Germany); the detection was performed at 511 nm, using a diode array detector (DAD) (Hitachi L-2455). The solvents used (mobile phase) were A: H₂O/HCOOH (9:1), and B: H₂O/CH₃CN/HCOOH (6:3:1), in a gradient of 20–85% from solution B for 70 min at a flow rate of 1.0 mL/min. The column was then washed with 100% of solution B for 20 min. Before each use, the column was stabilized for the initial conditions for another 20 min [26].

Animals and experimental design

Four-week-old male Wistar rats were obtained from Charles River Laboratories (Barcelona, Spain), and maintained under standard conditions (temperature 24–25°C, humidity 70–75%, lighting regimen of 12 h light/dark cycle), in plastic cages with free access to water and pellet food. Animal welfare and experimental procedures were carried out in accordance to the European Union regarding animal experimentation (Directive of the European Counsel 86/609/EEC) and approved by the Portuguese National Authority for Animal Health (Direcção-Geral de Alimentação e Veterinária—DGAV). All efforts were made to minimize the animals suffering and to reduce the number of animals used. An early humane endpoint criteria was adopted: although weight loss was expected in this disease model, if this loss exceeded 20% of the initial weight, animals would be euthanized. The rats were randomly divided into four groups: (i) non-colitic control (n = 10); (ii) TNBS-colitic control (n = 10); (iii) TNBS-induced rats treated with ARF 10 mg.kg^-1 (n = 10); and (iv) TNBS-induced rats treated with 5-ASA 100 mg.kg^-1 (n = 10). The ARF and the therapeutic agent were administered solubilized in a mixture of 0.9% NaCl and 0.5% carboxymethylcellulose (vehicle), in a single dose by oral gavage, during 8 days after colitis induction by TNBS.

The dose of ARF used was chosen on basis of preliminary experiments, as the lowest to obtain safety and efficacy in the referred colitis rat model, and that of 5-ASA was as reported in literature [5,27] and taking into consideration the dose translation from animal to humans [28].

Induction of colitis

Colonic inflammation was induced as described by Siddiqui et al [29]. Rats were fasted overnight and were then anesthetized with ketamine (50 mg.kg^-1) and chlorpromazine (2.3 mg.kg^-1), to allow the rectal administration of TNBS. Briefly, the tip of a polyethylene catheter was advanced transanally 8 cm into the distal colon and a single dose of TNBS was instilled intraluminally (10 mg of TNBS dissolved in 0.25 mL of 50% ethanol) to induce colitis. The animals were maintained in a head-down position for approximately 60 seconds to prevent leakage of the infusate. Non-colitic control group was subjected to the same procedure, infusing a saline buffer instead of TNBS. After one day, the rats were treated for 8 days as assigned previously.

Macroscopic assessment and scoring of TNBS colitis severity

Rats were sacrificed by cervical dislocation under anaesthesia with ketamine (50 mg.kg^-1) and chlorpromazine (2.3 mg.kg^-1). The colon was excised, opened longitudinally and washed in saline solution. Afterwards, the colon segment was weighed and its length measured. Each colon was scored for macroscopically visible damage by two observers unaware of the treatment, according to the criteria reported by Bell et al [30] and described in (Table 1). Representative whole gut specimens were taken from the inflamed colon region, or its equivalent segment in the control group, and stored at -80°C for subsequent biochemical measurements.

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Table 1. Criteria for the colonic macroscopic damage score assessment.

https://doi.org/10.1371/journal.pone.0174116.t001

Myeloperoxidase activity

Colonic mucosa was assayed for MPO activity as described by Stucchi et al [31], with slight modifications. Samples excised from each animal were thawed, and approximately 30–50 mg of mucosa was homogenized on ice with a Polytron tissue homogenizer in 4 ml of ice-cold 5 mM phosphate buffer (pH 6.0). To remove haemoglobin and other blood products that could interfere with this assay, the homogenate was centrifuged at 30000g, for 30 min, at 4°C and the supernatants discarded and the pellet resuspended in phosphate buffer, for three times. Finally, the pellet was solubilized in 10 volumes of ice-cold hexadecyltrimethylammonium bromide (0.5%) in phosphate buffer (50 mM, pH 6.0) and subjected to three cycles of freezing/thawing to extract the enzyme. The extract was allowed to stand at 4°C for 20 min and then centrifuged at 12500g for 15 min at 4°C. MPO activity was evaluated in the supernatant, by mixing 10 μL of this supernatant with 2.99 mL of 50 mM phosphate buffer, pH 6.0, containing 0.167 mg.mL^-1 of o-dianisidine dihydrochloride and 0.0005% of H₂O₂. The absorbance decrease of the reaction mixture was monitored at 460 nm for 2 min. Results were expressed as U MPO.mg^-1 tissue, being one unit of MPO activity defined as the amount of enzyme that degrades 1 μmol of hydrogen peroxide per minute.

Alkaline phosphatase activity

ALP activity was measured in colon tissue samples by the method described by Bessey et al. [32] as modified by Sanchez et al. [33]. The samples were homogenized in cold saline solution (1:20 w/v) and centrifuged at 7000g for 10 min at 4°C. The supernatants were used to determine spectrophotometrically the mucosal ALP activity, by mixing 100 μL of each sample with 1 mL of glycine (50 mM, pH 10.4), containing 5.5 mM p-nitrophenylphosphate and 0.5 mM magnesium chloride. After incubation for 30 min at 37°C, 10 mL of 0.02 M sodium hydroxide were added to stop the enzymatic reaction, and the p-nitrophenol formed was measured at 405 nm. The protein content was determined by the Bradford reaction using the Bio-Rad protein assay dye reagent (Bio-Rad, Hercules, California, USA), to express ALP activity as mU. g^-1 of protein. One unit of ALP activity is defined as the amount of enzyme that catalyzes the transformation of one micromole of substrate per minute.

Measurement of GSH/GSSG ratio

Total glutathione and GSSG were quantified in colon samples by an enzymatic recycling assay, essentially as described by Griffith et al [34]. The colon samples were previously treated by homogenization in extraction buffer containing 0.1% Triton X-100, 0.6% sulfosalicylic acid, 0.1 M KH₂PO₄ and 5 mM Na₂PO₄, pH 7.5), followed by centrifugation at 3000g, at 4°C, for 10 min [35]. Total glutathione (GSH + GSSG) was assessed in the supernatant in a 96-well plate. Briefly, 20 μL of supernatant was added to 120 μL of freshly prepared 5 mM DTNB plus glutathione reductase (1:1 v/v) in 0.1 M potassium phosphate buffer and 60 μL of 2.4 mM β-NADPH, also prepared in the same phosphate buffer. The absorbance due to the yellow dianion formed by the reaction of thiol groups and DTNB, was immediately read at 412 nm, using a Synergy HT plate reader (Bio-Tek Instruments) and followed for 2 min, with reading intervals of 30 sec. For the GSSG determination, the procedure was similar but prior to the assay, the GSH was blocked by derivatization using 2-vinilpyridine, by incubating 100 μL of the tissue samples with 2 μL of this masking agent and 6 μL of triethanolamine, during 1 h at room temperature, in a fume hood. Colon glutathione content (total and oxidized) was calculated using concurrently run standard curves in nmol per mg of cellular protein, and expressed as GSH/GSSG ratio.

Measurement of glutathione peroxidase activity

The activity of GPX in colon samples was evaluated using a colorimetric assay kit purchased from Abcam (Cambridge, UK), which monitors GSH oxidation by recording the consumption of NADPH at 340 nm. Colonic tissue extraction and enzymatic activity were performed in accordance to the manufacturer’s protocols and the results expressed in U per gram of colonic tissue.

Western-blot analysis of MPO, COX-2 and iNOS expressions

Colonic tissues were processed according to the method described by Sanchez-Fidalgo et al. [36] slightly modified. Briefly, frozen colonic tissues were weighed and homogenized in ice-cold lysis buffer (50 mM Tris–HCl, pH 8; 150 mM NaCl; 0.1% Triton X-100; 0.1% protease inhibitor cocktail; 1 mM PMSF; 0.5 mM EDTA; and 8 mM MgCl₂). Homogenates were incubated at 4°C for 2 h with stirring, and then cell debris were removed by centrifugation (12000g, 20 min, at 4°C) and the supernatants (cytoplasmic extracts) were collected and stored at -80°C until use. Protein concentration was determined using the Bio-Rad protein assay kit. Aliquots of the supernatant, containing equal amount of reduced and denaturated proteins (80 μg), were separated by SDS/PAGE electrophoresis in a 10% (v/v) acrylamide gel and further transferred onto polyvinylidene difluoride (PVDF) membranes (Amersham Biosciences, UK) by electroblotting, using the Trans-Blot Turbo Transfer System of Bio-Rad (Hercules, California, USA). The membranes were blocked with skimmed milk in TBS-T buffer (20 mM Tris-HCl, 150 mM NaCl, 0.1% Tween) to avoid non-specific binding. Afterwards the membranes were probed overnight, at 4°C, with specific primary antibodies against MPO, COX-2, iNOS and β-actin. Each membrane was then washed three times with TBS-T and incubated with the respective alkaline phosphatase-conjugated secondary antibodies, for 1 h, at room temperature. Immunodetection was performed by chemifluorescence after blots exposition to enhanced chemifluorescent reagent in a Typhoon 9000 scanner (Amersham Biosciences, UK) and analysed with the ImageQuant^TM software from Amersham Biosciences (UK). β-Actin was used as control for protein loading.

Statistical analysis

All results are expressed as the mean ± S.E.M. of at least 8 animals per group, and each sample assayed in duplicate. Differences between means were tested for statistical significance using a one-way or two-way analysis of variance (ANOVA), using Dunnett’s multiple comparisons test as post hoc test. All statistical analysis was carried out with the GraphPad Prism version 5 (GraphPad Software, Inc., CA, USA) and values of P < 0.05 were accepted as statistically significant.

The blueberry extract showed a high content and a great diversity of anthocyanins

Anthocyanin analysis of the anthocyanin-rich fraction showed a high content of anthocyanins, about 10.28 ± 0.48 g/L, or 98.75 ± 5.71 mg/100g of fruit, in terms of malvidin-3-glucoside. The total phenolic content of this fraction was 12.92 ± 1.59 g/L, or 119.96 ± 14.80 mg/100g of fruit, in terms of gallic acid equivalents. Moreover, using HPLC-DAD we could confirm that this fraction showed also a wide variety of anthocyanin molecules (15 peaks detected) as shown in Fig 1. The anthocyanins detected were, in descending order of amount, malvidin, petunidin, peonidin, delphinidin and cyanidin, conjugated with either galactose, glucose or arabinose, being malvidin-3-galactoside (20.93%) and petunidin-3-arabinoside (18.70%) the main anthocyanins detected (Fig 1 inset).

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Fig 1. HPLC-DAD chromatogram of blueberry anthocyanin-rich fraction.

The peak identification and the contents of the different anthocyanins are indicated in the inset table.

https://doi.org/10.1371/journal.pone.0174116.g001

The anthocyanin-rich fraction improved more efficiently than 5-ASA the recovery of body weight and the macroscopic colonic damage in TNBS-induced colitis in rats

During the study, the animals were constantly monitored for variations in body weight and general health. The inflammatory status in the TNBS-colitis control group was associated with severe anorexia and diarrhea, when compared to non-colitic control. Accordingly, as shown in Fig 2A, TNBS-colitis control group showed no significant weight gain with time, in contrast with the weight gain observed in healthy rats (115.7 ± 2.0%). Rats treated with ARF exhibited a significant recovery along the time, when compared with TNBS-colitis control group and the extent of recovery was clearly and statistically higher than that provided by 5-ASA, especially in the last two days. Notice that the observed benefits occurred at a concentration of anthocyanins about 30 times lower than that of 5-ASA (10 mg.kg^-1 of ARF corresponds to 0.02 mmol.kg^-1 in terms of malvidin-3-glucoside, while 100 mg.kg^-1 of 5-ASA corresponds to 0.65 mmol.kg^-1).

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Fig 2. Effect of anthocyanin-rich fraction, as compared with 5-ASA, on body weight and on macroscopic colonic damage in rats with TNBS-induced colitis.

After colitis induction, each group of animals was treated daily for 8 days with either ARF or 5-ASA and their effects on body weight were recorded overtime and expressed in terms of % of the initial weight (A). After colon collection (day 8 post TNBS-induced colitis), macroscopic colitis severity was blindly assessed and characterized in terms of damage score (B). Values are mean ± SEM of at least 8–9 animals per group. ***P<0.001 vs non-colitic control; ^#P<0.05, ^##P<0.01, ^###P<0.001 vs TNBS-colitic control; ^§P<0.05 vs 5-ASA group.

https://doi.org/10.1371/journal.pone.0174116.g002

By the end of the experiment, the mortality in the TNBS-colitis control group was found to be very small (1/10), compared with the healthy, non-colitic control (0/10), indicating that the induced colonic injury was not fatal within 8 days, and neither the ARF nor 5-ASA, in the doses used, increased it. Additionally, neither TNBS nor the different treatments caused significant changes in the relative weights of the main organs (% of total body weight), such as liver, kidneys and heart (S1 Table) which are highly susceptible to drugs toxicity.

The intracolonic administration of TNBS in ethanol induced colonic inflammation which was eight days later characterized by several events, namely: i) severe necrosis of the mucosa, typically extending 4–6 cm along the colon; ii) bowel wall thickening; iii) colon shortening; iv) hyperemia; and v) focal adhesions to adjacent organs, according to the scale represented in Table 1. Altogether, these data were correlated for each group of animals and shown in Fig 2B, indicating that the treatment with ARF counteracted the TNBS-induced damage score in a more efficient way than with 5-ASA. ARF also led to a very strong decrease in the colonic weight/length ratio (Fig 3A), being even more effective than 5-ASA, although in a much lower molar concentration than this drug. Representative colon pictures of each group are shown in Fig 3B.

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Fig 3. Effect of anthocyanin-rich fraction, as compared with 5-ASA, on the colon weight/length ratio of TNBS-induced colitic rats.

On day 8, post TNBS-induced colitis, the colon of each animal was excised and evaluated in terms of weight and length. The colon weight vs length ratio for each group of animals is represented in graph A. Representative images of typical colons of each group are also shown (B). Values are mean ± SEM of at least 8–9 animals per group. ***P<0.001 vs non-colitic control; ^##P<0.01, ^###P<0.001 vs TNBS-colitic control.

https://doi.org/10.1371/journal.pone.0174116.g003

The anthocyanin-rich fraction inhibited the amount of active myeloperoxidase and the alkaline phosphatase activity, more efficiently than 5-ASA

The beneficial effects of our anthocyanin extract on TNBS-induced rat colitis were also studied biochemically in terms of well-established inflammatory markers. For this purpose, we analysed the MPO activity and its protein expression in colon sections from the different groups of rats, by the end of the experiment. The activity of this enzyme has been widely accepted as a strong marker of the inflammation degree, in terms of leukocyte infiltration in tissues [31]. As shown in Fig 4, TNBS led to a significant increase in either MPO activity (A) or its protein expression (B), when compared with the non-colitic control rats. Treatment with ARF, along 8 days after colitis induction, reduced significantly MPO activity (Fig 4A) and its protein expression (Fig 4B) in a higher extent than with 5-ASA, indicating a higher anti-inflammatory action.

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Fig 4. Effect of anthocyanin extract administration on colon myeloperoxidase activity and expression as compared with 5-ASA, in TNBS-induced colitis.

MPO activity (A) was measured in colon tissue homogenates and expressed in units of enzyme activity per mg of tissue. MPO protein expression (B) was assessed in colon tissue samples by Western blotting and expressed as fold increase relative to the non-colitic control group. Values are mean ± SEM from at least 8–9 animals per group, each one in duplicate. ***P<0.001 vs non-colitic control; ^#P<0.05, ^##P<0.01, ^###P<0.001 vs TNBS-colitic control.

https://doi.org/10.1371/journal.pone.0174116.g004

Furthermore, we determined the ALP activity, since it has also been reported as a sensitive marker of inflammation in the intestine [33]. Results are shown in Fig 5 and also indicated a significant capacity of anthocyanins to reduce this enzyme activity, in contrast with 5-ASA, whose effect was not statistically significant.

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Fig 5. Effect of anthocyanin extract administration on colon alkaline phosphatase activity, as compared with 5-ASA, in TNBS-induced colitis.

ALP activity was measured in colon tissue homogenates and expressed in units of enzyme activity per g of protein. Values are mean ± SEM from at least 8–9 animals per group, each one in duplicate. **P<0.01 vs non-colitic control; ^#P<0.05, vs TNBS-colitic control.

https://doi.org/10.1371/journal.pone.0174116.g005

The colonic antioxidant defenses were improved by the anthocyanin-rich fraction, more efficiently than by 5-ASA

An imbalance in the production of different reactive oxygen species, which may overwhelm the tissue antioxidant defenses, can be another molecular event involved in IBD [37]. Thus, to probe the colonic redox status, we decided to evaluate GSH content and GPx activity. In the TNBS-colitic control group, a great decrease (by about 65%) in the colonic GSH/GSSG ratio (Fig 6A), as well as in the GPx activity (by about 88%) (Fig 6B) was observed. ARF treatment significantly counteracted the induced decrease in GSH/GSSG ratio, indicating an improvement in the host antioxidant defenses, whereas 5-ASA was devoid of a significant effect, in the same experimental conditions (Fig 6A). Similar results were obtained for GPX activity (Fig 6B), showing a higher efficacy of anthocyanin fraction in recovering the antioxidant defenses, as compared with 5-ASA.

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Fig 6. Effect of anthocyanin-rich fraction on colon GSH/GSSG ratio and GPX activity, as compared with 5-ASA, in TNBS-induced colitic rats.

GSH/GSSG ratio and GPx activity were determined in samples of colonic tissue of each animal, as described in Materials and Methods. Statistics of GSH/GSSG ratio (A) and of GPx specific activity (B) for each group of animals are presented. Values are mean ± SEM obtained from at least 8–9 animals per group, each one in duplicate. ***P<0.001 vs non-colitic control; ^#P<0.05, ^##P<0.01 vs TNBS-colitic control.

https://doi.org/10.1371/journal.pone.0174116.g006

The anthocyanin-rich fraction strongly counteracted TNBS-stimulated expression of colon COX-2 and iNOS enzymes

The colonic inflammatory status was also characterized by a significant increase in the colonic COX-2 and iNOS protein expressions, relative to non-colitic control, as ascertained by Western blotting analysis from homogenates of inflamed tissue (Fig 7). Treatments with either ARF or 5-ASA strongly down-regulated COX-2 expression (Fig 7A), reverting it to control levels. This indicates that COX-2 inhibition is a relevant action pathway for anthocyanins, like for 5-ASA. Concerning the effects on iNOS expression, only the treatment with ARF could counteract drastically its increase in TNBS-induced colitis (by about 95%) whereas 5-ASA, in the dose used, did not show a significant effect (Fig 7B).

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Fig 7. Comparison of the effects of anthocyanin-rich fraction and 5-ASA on COX-2 and iNOS protein expressions in colon tissue samples of colitic rats.

COX-2 (A) and iNOS (B) protein expressions were evaluated by Western blotting in each animal of each group and expressed as fold increase relative to the non-colitic control group. Values are means ± SEM from of at least 8–9 animals per group, each one in duplicate. ***P<0.001 vs non-colitic control; ^##P<0.01, ^###P<0.001 vs TNBS-colitc control; ^§§P<0.01 vs 5-ASA group.

https://doi.org/10.1371/journal.pone.0174116.g007