Oxidative neuronal cell damage has been implicated in the pathogenesis of neurodegenerative disorders such as Alzheimer's disease, Parkinson's disease and amyotrophic lateral sclerosis(Reference Le Forestier, Lacomblez and Meininger1–Reference Yacoubian and Standaert4). It is mediated by reactive oxygen species, including H2O2, superoxide anion and hydroxyl radicals, which are generated as by-products of normal and irregular metabolic processes. Reactive oxygen species attack cellular biomolecules and disrupt cellular function and membrane integrity, thereby leading to apoptosis(Reference Mancuso, Orsucci and Siciliano2, Reference Busija, Gaspar and Domoki5, Reference Cadet, Douki and Ravanat6). As a major component of reactive oxygen species, H2O2 induces apoptosis in many different cell types, and therefore, it has been extensively used as an inducer of oxidative stress in in vitro models(Reference Heo, Choi and Choi7–Reference Yang, Zhang and Huang9).
Exposure to reactive oxygen species from a variety of sources has led organisms to develop a series of defence mechanisms. Such mechanisms involve prevention, repair, physical defence and antioxidant defence. Non-enzymatic antioxidants are represented by glutathione, ascorbic acid (vitamin C), α-tocopherol (vitamin E) and carotenoids. Enzymatic antioxidant defence includes superoxide dismutase (SOD), glutathione peroxidase and catalase (CAT)(Reference Valko, Leibfritz and Moncol10). However, the effects of SOD may become deleterious when it is overexpressed because of the resulting H2O2 production(Reference Lindenau, Noack and Possel11).
The mitogen-activated protein kinase (MAPK) family plays a critical role in the cellular response to a wide range of stimuli. Indeed, the dynamic balance between branches of the MAPK family, namely extracellular signal-regulated kinase (ERK1/2), c-Jun N-terminal kinase (JNK) and p38 MAPK, is implicated in regulating cell death/survival(Reference Valko, Leibfritz and Moncol10, Reference Murphy and Blenis12). Several mechanisms are involved in the specificity of different, even opposing signals of the MAPK family, including (i) duration and strength of the signal, (ii) interaction with various scaffold proteins, (iii) subcellular localisation, (iv) presence of several isoforms, (v) extensive cross-talk and interplay between MAPK cascade and other pathways; (vi) post-translational modifications other than phosphorylation(Reference Krishna and Narang13). Furthermore, the spatial distribution and temporal qualities of MAPK can markedly alter the qualitative and quantitative features of downstream signalling to immediate early genes and the expression of immediate early genes-encoded protein products. As a result, immediate early gene products provide a molecular interpretation of MAPK dynamics, enabling the cell to program an appropriate biological response(Reference Murphy and Blenis12).
Natural antioxidants have been reported to play a major role in blocking oxidative stress induced by free radicals. Supplementation with fruits and vegetables rich in polyphenols is beneficial for both forestalling and reversing the deleterious effects of ageing on neuronal communication and behaviour(Reference Joseph, Shukitt-Hale and Lau14–Reference Shukitt-Hale, Carey and Jenkins17). The observed protection may be due to the antioxidant and anti-inflammatory properties of the polyphenolic compounds found in these fruits and vegetables(Reference Yang, Zhang and Huang9, Reference Ramassamy18–Reference Wang, Wen and Huang20).
Blueberries show the highest antioxidant capacity among all fruits and vegetables(Reference Wolfe, Kang and He21). Blueberries and their phenolic compounds, such as anthocyanins and flavonoids, have been identified as potential contributors of amelioration of neuronal cell dysfunction(Reference Duffy, Spangler and Devan22–Reference Lau, Bielinski and Joseph25). Biotransformation of blueberry juice with a novel strain of bacteria isolated from the blueberry flora and named Serratia vaccinii increases its phenolic content and antioxidant activity(Reference Martin and Matar26). It also modifies the biological activity of biotransformed blueberry juice (BJ), such as inhibiting NO production in macrophages(Reference Vuong, Martin and Matar27) and increasing its antiobesity and antidiabetic effects(Reference Vuong, Martineau and Ramassamy28, Reference Vuong, Benhaddou-Andaloussi and Brault29). The aim of the present study was to assess the neuroprotective property of BJ against H2O2-induced oxidative stress in cultured neuronal cells.
Materials and methods
Preparation of fermented blueberry juice
Mature lowbush blueberries (Vaccinium angustifolium Ait.) were purchased from Cherryfield Foods, Inc. (Cherryfield, ME, USA) as fresh and untreated fruits. Blueberry juice was extracted by blending the fruits (100 g) in a Braun Type 4259 food processor with an equivalent quantity (100 g) of Minimal Broth Davis without dextrose (Difco Laboratories, Detroit, MI, USA). The fruit mixture was then centrifuged at 500 g for 6 min to remove fruit skin and insoluble particles. The resulting juice was sterilised using 0·22 μm Express Millipore filters (Millipore, Etobicoke, ON, Canada).
Serratia vaccinii bacteria were cultured as described previously(Reference Martin and Matar26). The juice was inoculated with a saturated culture of Serratia corresponding to 2 % of the total juice volume. After a 4 d fermentation period, the transformed juice was sterilised by 0·22 μm filtration. The total phenolic content was then measured by the Folin–Ciocalteau method using gallic acid as the standard, and hence expressed as μm gallic acid equivalent. The total phenolic content was increased from 4581 to 19 338 μm-gallic acid equivalent, confirming successful transformation. Normal blueberry juice (NJ) and BJ have been partially characterised as described elsewhere(Reference Martin and Matar26, Reference Matchett, MacKinnon and Sweeney30).
Cell culture
Murine N2a neuroblastoma cell line was obtained from the American Type Cell Collection (Chicago, IL, USA). Cells were cultured in minimum essential medium containing fetal bovine serum (10 %, v/v; Sigma-Aldrich, Oakville, ON, Canada) and penicillin/streptomycin (0·05 mg/ml) at 37°C in a humidified atmosphere with 5 % CO2 in twenty-four-well plates for viability and toxicity experiments, twelve-well plates for SOD activity experiments and six-well plates for enzyme activity and signalling experiments.
Viability and toxicity assay
Cell viability was assessed by water-soluble tetrazolium salt-1 (WST-1) assay (Roche, Laval, QC, Canada). Briefly, after pretreatments with blueberry juices, H2O2 was added at a final concentration of 0·75 mm for 24 h. WST-1 was added (10 %, v/v) and incubated at 37°C for 2 h. The absorbance was measured at 450 nm in a plate reader (Wallac Victor 2; Perkin-Elmer, St-Laurent, QC, Canada).
In preliminary experiments, H2O2 induced a 30–35 % cell loss at 0·75 mm. This concentration was used for all the experiments thereafter. The protective effect of BJ was maximised if cells were pretreated with BJ for 1 h before adding H2O2.
Cell toxicity was measured by lactate dehydrogenase assay (Roche). After treatments, 100 μl of the culture medium were transferred to a ninety-six-well plate. Cells were lysed with 0·1 m-NaOH for 10 min on ice, and 100 μl of lysate were transferred to a ninety-six-well plate. One hundred microlitres of assay mixture were added to each well, and incubated at room temperature for 10 min. The absorbance was measured at 450 nm.
GSH:GSSG ratio
GSH:GSSG ratio was measured using BIOXYTECH GSH/GSSG-412™ kit (OxisResearch™, Foster City, CA, USA). After treatments, cells were placed on ice and washed twice with ice-cold Krebs phosphate buffer. Twenty microlitres of scavenger were added to GSSG sample, while 20 μl of buffer were added to GSH sample. Cells were then lysed in 200 μl of lysis buffer (50 mm-Tris–HCl (pH 7·5)/0·5 % Triton X-100). Lysed cells were scraped and transferred to microcentrifuge tubes. Samples were allowed to lyse for an additional 15 min on ice with periodic vortexing. The lysates were centrifuged at 300 g at 4°C for 10 min, and the samples were used for determination of GSH:GSSG ratio according to the manufacturer's instructions.
Enzymatic activity assay
SOD enzyme activity was measured using the SOD Assay Kit-WST (Dojindo Molecular Technologies, Inc., Gaithersburg, MD, USA). After treatments, cells were placed on ice and washed twice with ice-cold Krebs phosphate buffer. Cells were lysed in 200 μl of lysis buffer (50 mm-Tris–HCl (pH 7·5)/0·5 % Triton X-100). Lysed cells were then scraped and transferred to microcentrifuge tubes. Samples were allowed to lyse for an additional 15 min on ice with periodic vortexing. The lysates were centrifuged at 300 g at 4°C for 10 min, and 20 μl of this sample solution were used for determination of SOD enzyme activity according to the manufacturer's instructions. CAT activity was determined by adding 900 μl of 30 mm-H2O2 to 100 μl of the cell lysate. The disappearance of H2O2 was monitored at 240 nm for 1 min.
Western blot analysis
After treatments, cells were placed on ice and washed three times with ice-cold Krebs phosphate buffer. Cells were lysed in radioimmunoprecipitation assay lysis buffer (50 mm-HEPES, pH 7·4, 150 mm-NaCl, 5 mm-EDTA, 2 mm-MgCl2, 1 % Triton X-100, 1 % sodium deoxycholate and 0·1 % SDS) containing protease inhibitors (2 mm-phenylmethylsulphonyl-flouride and Complete Mini protease inhibitor cocktail tablets (Roche)) and phosphatase inhibitors (0·5 mm-NaF, 2 mm-sodium orthovanadate and 1 mm-sodium pyrophosphate). Lysed cells were then scraped and transferred to microcentrifuge tubes. Samples were allowed to lyse for an additional 15 min on ice with periodic vortexing. Lysates were then centrifuged at 4500 g, and supernatants were collected and stored at − 80°C until further analysis.
Protein concentration of lysates was assessed using the bicinchoninic acid colorimetric method (Pierce, Rockford, IL, USA) according to the manufacturer's instructions. From each sample, 120 μg of total protein were loaded onto an 8 % acrylamide gel, and were separated at 4°C for 3 h at 75 mA, followed by 15 h at 20 mA, using a Protean II electrophoresis apparatus (BioRad, Missisauga, ON, Canada). Separated samples were then electrotransferred onto polyvinylidene fluoride membranes (Millipore) at 4°C for 90 min at 1 A using a Transblot apparatus (BioRad). Membranes were stained with Ponceau red solution (5 %, in acetic acid; Sigma) and photographed, and were then washed in Tris-buffered saline Tween-20 (TBST, 50 mm-Tris, pH 7·4, 150 mm-NaCl and 0·5 % Tween-20) followed by blocking in TBST +5 % non-fat dried milk for 1 h at ambient temperature. Membranes were incubated overnight at 4°C with the following antibodies: rabbit anti-phospho-mitogen-activated protein kinase/extracellular signal-regulated kinase kinase (MEK1/2; Ser217/221), rabbit anti-phospho-p38 MAPK (Thr180/Tyr182), mouse anti-phospho-ERK1/2 (Thr202/Tyr204) and rabbit anti-phospho-stress-activated protein kinase (SAPK)/JNK (Thr183/Tyr185) (cat #9121, #9211, #4377, #9251, respectively; Cell Signaling Technology, Incorporation, Danvers, MA, USA) at 1:1000 dilution in TBST +5 % bovine serum albumin. Membranes were then incubated for 60 min at ambient temperature with horseradish peroxidase-conjugated anti-rabbit or anti-mouse secondary antibodies (Jackson Immunoresearch Laboratories, Incorporation, West Grove, PA, USA) at 1:100 000 dilution in TBST +5 % milk. After washing with TBST, the blots were revealed using the enhanced chemiluminescence method (Amersham, Piscataway, NJ, USA) on a blue-light-sensitive film (Amersham). Densitometric analysis was performed using a Hewlett-Packard flatbed scanner and NIH software Image J 1.37v.
Statistical analysis
Statistical analysis of the data by two-way ANOVA and Fisher's post hoc tests was performed using StatView software (Cary, NC, USA). Statistical significance was set at P ≤ 0·05. Data are reported as mean values with their standard errors.
Results
Biotransformed blueberry juice protects neurons against hydrogen peroxide-induced cell death
To investigate the potential protective effects of blueberry juices in vitro, N2a neuroblastoma cells were treated with H2O2 in their presence or absence. H2O2 alone induced significant loss of cell viability in a dose-dependent manner (data not shown), whereas sterile BJ or NJ alone were non-toxic. Co-treatment with BJ significantly protected neurons against H2O2-induced oxidative stress in a dose-dependent manner, and completely abolished H2O2 toxicity from a concentration of 30 μm-gallic acid equivalent onwards, whereas NJ did not show any effect (Fig. 1).
Because the WST-1 assay is based on mitochondrial activity and the latter can be affected by plant polyphenolic compounds(Reference Sun, Wang and Simonyi31), we confirmed the present results with the lactate dehydrogenase assay. Again, H2O2 induced dose-dependent neuronal cell death that was countered by BJ but not by NJ (Fig. 2).
Biotransformed blueberry juice preserves GSH/GSSG balance
Neither NJ nor BJ alone affected the GSH:GSSG ratio, whereas H2O2 significantly decreased GSH:GSSG ratio by 19 % after 30 min and by 21 % after 4 h. However, H2O2 significantly lost its tendency to reduce the GSH:GSSG ratio in BJ-pretreated neurons, while no significant difference was observed in NJ-pretreated cells (Fig. 3).
Biotransformed blueberry juice increases catalase and superoxide dismutase activities
When administered alone, BJ increased CAT activity in N2a cells. CAT activity reached the highest level after a 4 h treatment (0·13 (sem 0·02) v. 0·09 (sem 0·01) mm/min per mg protein, 4 v. 0 h, P < 0·05), and then gradually decreased towards control values (Fig. 4). In contrast, control and NJ-treated cells displayed a rather stable CAT activity over the 24 h experimental period. When H2O2 alone was added, CAT activity increased rapidly and reached the highest level after 24 h (0·13 (sem 0·02) v. 0·08 (sem 0·01) mm/min per mg protein, H2O2v. control at 24 h, P < 0·05). Neither BJ nor NJ treatment could significantly affect H2O2 actions even though BJ treatment had lowered H2O2-increased CAT activity (Fig. 4).
BJ, but not NJ, rapidly and significantly increased SOD activity when administered alone (Fig. 5). However, SOD activity returned to the basal level after 24 h. H2O2 by itself gradually increased SOD activity. SOD activity reached the highest level after 4 h, and then remained constant at this level. When H2O2 was added to BJ-treated cells, SOD activity was slightly increased, and then returned to the basal level after 24 h (Fig. 5). As for CAT, NJ pretreatment did not show any effect (data not shown).
Biotransformed blueberry juice protection is associated with the activation of c-Jun N-terminal kinase and mitogen-activated protein kinase p38
Exposure of N2a cells to BJ alone triggered the activation of both p38 MAPK (Fig. 6) and JNK (Fig. 7), while NJ did not show any effect compared with the vehicle control. BJ induced maximal phosphorylation of p38 MAPK by 90 % after 30 min (Fig. 6), and of JNK by 66 % after 2 h (Fig. 7). While H2O2 did not modify JNK phosphorylation (Fig. 7), it increased p38 MAPK activity by 111 % after 30 min, which then gradually decreased to a very low level after 4 h (19 % of time 0 control, Fig. 6). In BJ-treated cells challenged with H2O2, p38 MAPK and JNK activities followed the same pattern observed in cells treated with BJ alone, albeit at a slightly lower level, hence indicating a significant dampening of H2O2 effects (Figs. 6 and 7). For both enzymes, NJ treatment gave results indistinguishable from those observed for vehicle control or H2O2 groups, respectively (data not shown).
Biotransformed blueberry juice inhibition of hydrogen peroxide toxicity is associated with the protection of mitogen-activated protein kinase/extracellular signal-regulated kinase kinase1/2 and extracellular signal-regulated kinase1/2 activities
Baseline MEK1/2 phosphorylation exhibited a gradual and steady decline within the 4 h experimental period, and this was not affected by either NJ or BJ treatments (Fig. 8). In contrast, ERK1/2-activated state remained stable in control and NJ- and BJ-treated groups (Fig. 9). When H2O2 was added to N2a cells, MEK1/2 and ERK1/2 phosphorylations were rapidly and significantly decreased by half within 30 min (Figs. 8 and 9). ERK1/2 then gradually increased to the initial level by 2 h, while MEK1/2 remained stable at its new low level. In BJ-treated cells, there were no significant changes in MEK1/2 and ERK1/2 activities induced by H2O2 (Figs. 8 and 9).
Discussion
Blueberry and blueberry products have been demonstrated to possess the potential to reduce age-related neurodegeneration and to enhance motor and cognitive functions(Reference Joseph, Shukitt-Hale and Lau14, Reference Shukitt-Hale, Carey and Jenkins17). Our group has discovered a bacterium from the blueberry flora that can biotransform blueberry juice(Reference Martin and Matar26). This greatly accentuates its antioxidant potential(Reference Martin and Matar26, Reference Seeram, Aviram and Zhang32), and endows it with novel anti-inflammatory(Reference Vuong, Martin and Matar27) and antidiabetic(Reference Vuong, Martineau and Ramassamy28, Reference Vuong, Benhaddou-Andaloussi and Brault29) biological activities. In the present study, we sought to explore the effect of such a biotransformation on the neuroprotective potential of blueberry juice. We chose H2O2 as a source of oxidative stress because it is formed endogenously as a natural by-product of enzymatic oxidase action or as a product of the dismutation of superoxide anion catalysed by SOD(Reference Pratico3). It contributes to the background level of cellular oxidative stress(Reference Fatokun, Stone and Smith33). It is generally accepted that the antioxidant enzymes CAT and glutathione peroxidase can protect cells from the effects of basal H2O2 production(Reference Fourquet, Huang and D'Autreaux34). The administration of exogenous H2O2 can elevate oxidative stress beyond the protective capacities of endogenous antioxidant defence systems, resulting in apoptosis or necrosis of cultured neurons(Reference Whittemore, Loo and Watt35).
We also chose murine neuroblastoma cells of the N2a line because they have been widely employed to investigate the antioxidant mechanisms involved in neurotoxicity, neuroprotection and neuronal repair(Reference Pizarro, Yeste-Velasco and Rimbau8, Reference Filiz, Caragounis and Bica36, Reference Kemmerling, Munoz and Muller37). In the present study, H2O2 (0·75 mm) caused a significant decrease in cell viability (35 %), but pretreatment of N2a cells with BJ blocked this oxidative stress-induced cytotoxicity in a dose-dependent manner. Similar protection was not found with NJ.
One of the first-line defence mechanisms against H2O2-induced toxicity is the antioxidant enzyme CAT. We found that BJ treatment alone significantly increased CAT activity by 44 %, and this was consistent with the parallel protection of neuronal cells against oxidative stress attack by H2O2. The mechanism through which BJ increased CAT activity is unknown. However, since the increase in CAT activity in BJ-treated neurons required at least 4 h to be fully expressed, BJ might act via both transcriptional and translational mechanisms.
Another important enzymatic antioxidant defence mechanism involves SOD. Indeed, upregulation of SOD activity has been associated with neuroprotective capabilities in certain studies(Reference Kolla, Wei and Richardson38). However, since SOD-catalysed reactions also elevate endogenous H2O2, overexpression of SOD can also cause deleterious effects(Reference Lindenau, Noack and Possel11). In fact, excessive H2O2 production caused by SOD overexpression has been implicated in the brain injury observed after perinatal hypoxia–ischaemia(Reference Ditelberg, Sheldon and Epstein39). In our study, H2O2 clearly increased SOD activity, which was maintained at a high level over 24 h. This may appear paradoxical, but it could simply be indicative of the state of oxidative stress induced in neuronal cells by our experimental conditions. When cells were pretreated with BJ, however, the rise that H2O2 induced in SOD activity was blunted, and the activity returned to normal levels within 24 h. These results further support the notion that BJ protected neurons from H2O2-induced oxidative stress.
Apart from enzymatic antioxidant system, non-enzymatic protective mechanisms exist, one of the most important being the GSH:GSSG system(Reference Valko, Leibfritz and Moncol10). In our experimental conditions, GSH:GSSG ratio was reduced by H2O2 treatment, as expected if oxidative stress overcomes the capacity of this antioxidant system. In cells pretreated with BJ, this reduction of GSH:GSSG ratio was lost. Surprisingly, BJ alone did not modulate the GSH:GSSG ratio, and similarly, it had no impact on GSH production (data not shown). One can speculate that GSH reductase and GSH peroxidase activities have been modulated by BJ, and further studies are necessary to address this point. Nonetheless, it is well known that phenolic compounds, such as quercetin, epicatechin, mangiferin, patuletin, nepetin, and axillarin, can increase both GSH reductase and GSH peroxidase activities(Reference Mahakunakorn, Tohda and Murakami40–Reference Kim, Park and Lee42).
Although H2O2 has been widely used to study the underlying molecular mechanisms of neurotoxicity and neuroprotection in N2a cells, detailed information on the cell death pathways involved is still lacking, notably at the level of the three branches of the MAPK family, namely ERK1/2, JNK, and p38 MAPK. The present study investigated the kinetics of these members of the MAPK family after H2O2 challenge. To our knowledge, this has not been reported previously in the N2a cell system.
We found that H2O2 first induced a transient inactivation of both JNK and ERK1/2 while increasing p38 MAPK activity within 30 min. Then, ERK1/2 activity gradually returned to basal levels by 4 h, whereas both JNK and p38 MAPK activities were decreased to exhibit prolonged inactivation after 4 h. Both transient activation of p38 MAPK and prolonged activation of ERK1/2 have been correlated with H2O2-induced neurotoxicity in PC12 cells(Reference Wu, Zheng and Cui43, Reference Colognato, Laurenza and Fontana44).
The mechanisms by which H2O2 decreased both JNK and ERK1/2 phosphorylations are unknown. However, since MEK1/2 phosphorylation was also observed to decrease, this inactivation may be regulated by phosphatases with or without cross-talk between MAPK pathways. Recently, dual-specificity phosphatases, generally termed MAPK phosphatases, were found to control the spatiotemporal regulation of ERK1/2 and cross-talk between MAPK pathways(Reference Caunt, Armstrong and Rivers45). Further studies are necessary to clarify the involvement of MAPK phosphatases in the effects observed herein.
NJ did not show any effect on either basal or H2O2-induced MAPK member phosphorylations, and results were generally similar to the respective controls. In contrast, pretreatment with BJ rapidly increased basal p38 and JNK phosphorylations, which remained elevated for up to 4 h. Conversely, BJ did not have any influence on the basal behaviour of MEK1/2 or ERK phosphorylation observed in vehicle controls over the 4 h experimental period. In general, BJ significantly reduced the initial changes in the MAPK family member phosphorylation state described earlier after treatment with H2O2. Therefore, modifications in MAPK family enzymes appear to contribute to the protection of neurons against H2O2-induced cell death afforded by BJ. Indeed, although the role of JNK and p38 MAPK in apoptosis has been established in some cell lines, they have also been shown to contribute to survival, development and differentiation depending on their active isoform(Reference Krishna and Narang13). For examples, JNK1 and JNK2 were initially believed to possess redundant functions; however, it was found that JNK1 preferentially mediates apoptosis, whereas JNK2 is associated with cellular proliferation(Reference Nitta, Chu and Wong46). Similarly, MAPK p38α and p38β are involved in apoptosis, whereas MAPK p38γ and p38θ are more effective in cell survival(Reference Gutierrez-Sanmartin, Varela-Ledo and Aguilera47, Reference Lin, Mak and Yang48). Further studies are needed to address the involvement of p38 MAPK and JNK isoform stimulation and ERK1/2 inactivation in the neuroprotective effect of BJ. For instance, in the case of H2O2-induced inactivation of MEK1/2 and ERK1/2, BJ could have prevented these effects of the oxidant stress by blocking MAPK activity; future studies should address this possibility.
One of the first hypotheses that come to mind to explain the neuroprotective action of BJ relates to direct antioxidant mechanisms(Reference Dinkova-Kostova and Talalay49). Indeed, the total phenolic content in BJ was increased more than four times compared with NJ, with such compounds being well known for their antioxidant potential(Reference Martin and Matar26). For example, epigallocatechin-3-gallate, a phenolic compound from green tea, was recently found to accumulate in the mitochondria where it acts locally as a free radical scavenger to protect neurons(Reference Schroeder, Kelsey and Doyle50). In view of the heightened content in BJ, such an accumulation of phenolic compounds in the mitochondria may have been enhanced, with an expected increase in the free radical-scavenging capacity to protect neurons against oxidative stress. Moreover, the biotransformation of blueberry juice not only increases its phenolic content, but also produces novel compounds(Reference Martin and Matar26). Given that BJ was added at a gallic acid equivalent that was equal to that of NJ, one interesting possibility is that these novel compounds possess more potent antioxidant properties that could have contributed to protect neurons, as opposed to components of NJ. This hypothesis should be tested once the novel bioactive compounds in BJ are identified.
Another hypothesis to explain the observed BJ neuroprotective activity is the pro-oxidant hypothesis(Reference Halliwell51). Indeed, some phenolic compounds present in BJ may act as weak oxidants, thereby activating antioxidant defence mechanisms as observed herein for CAT(Reference Halliwell52). If neuronal cells defence systems were so prepared by BJ before H2O2 was added, H2O2-induced deleterious effects may thus have been inhibited. However, the pro-oxidant hypothesis also raises a limitation in our study. Indeed, some phenolic compounds, such as EGCG, can be oxidised in culture media, and form H2O2(Reference Halliwell51). Therefore, neurons pretreated with BJ and NJ may have been exposed to concentrations of H2O2 greater than that expected based on the amounts added in our experimental protocols. However, this increased H2O2 concentration does not appear to have had a significant deleterious impact because H2O2-induced cell death did not increase in NJ or BJ groups. On the contrary, if anything, such considerations only further highlight the significant beneficial neuroprotective effect of BJ, which may well be related to the changes in blueberry juice composition after the biotransformation.
In summary, the results of the present study indicate that BJ possesses a strong neuroprotective potential against H2O2-induced oxidative stress in the N2a neuronal cell line in vitro. BJ increased antioxidant enzyme activity as well as p38 MAPK and JNK activation while blocking H2O2-induced ERK1/2 activity modifications. We speculate that it is a combination of these various actions of BJ that contributed to protect neurons against cell death induced by oxidative stress. Although the active principles and their precise mechanisms of action remain to be identified, BJ may represent a promising approach to prevent and treat neurodegenerative disorders, and it may represent a source of novel therapeutic agents against these diseases.
Acknowledgements
The present study was funded by the Canadian Institutes of Health Research, Atlantic Innovation Funds, Atlantic Canada Opportunities Agency and Institute of Nutraceuticals and Functional Foods, a Strategic Research Group of the Quebec ‘Fonds de recherche sur la nature et les technologies’. T. V. conducted all the experiments, performed data analysis and drafted the paper. C. M., C. R., P. S. H. supervised and provided technical support for the study and revised the manuscript. The authors have no conflict of interest.