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Protective effect of serotonin derivatives on glucose-induced damage in PC12 rat pheochromocytoma cells

Published online by Cambridge University Press:  14 September 2009

Rosaria Piga*
Affiliation:
Department of Inflammation and Immunology, Graduate School of Medical Science, Kyoto Prefectural University of Medicine, Kamigyo-ku, Kyoto, Japan
Yuji Naito
Affiliation:
Department of Medical Proteomic, Graduate School of Medical Science, Kyoto Prefectural University of Medicine, Kamigyo-ku, Kyoto, Japan
Satoshi Kokura
Affiliation:
Department of Biomedical Safety Science, Graduate School of Medical Science, Kyoto Prefectural University of Medicine, Kamigyo-ku, Kyoto, Japan
Osamu Handa
Affiliation:
Department of Biomedical Safety Science, Graduate School of Medical Science, Kyoto Prefectural University of Medicine, Kamigyo-ku, Kyoto, Japan
Toshikazu Yoshikawa
Affiliation:
Department of Inflammation and Immunology, Graduate School of Medical Science, Kyoto Prefectural University of Medicine, Kamigyo-ku, Kyoto, Japan
*
*Corresponding author: Dr Rosaria Piga, fax +81 75 252 3721, email rosariapiga@tiscali.it
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Abstract

Oxidative damage is believed to be associated with ageing, cancer and several degenerative diseases. Previous reports have shown that safflower-seed extract and its major antioxidant constituents, serotonin hydroxycinnamic amides, possess a powerful free radical-scavenging and antioxidative activity, paying particular attention to atherosclerotic reactive oxygen species (ROS)-related dysfunctions. In the present report, we examined a still unknown cell-based mechanism of serotonin derivatives against ROS-related neuronal damage, phenomena that represent a crucial event in neurodegenerative diseases. Serotonin derivatives N-(p-coumaroyl)serotonin and N-feruloylserotonin exerted a protective effect on high glucose-induced cell death, inhibited the activation of caspase-3 which represents the last and crucial step within the cascade of events leading to apoptosis, and inhibited the overproduction of the mitochondrial superoxide, which represents the most dangerous radical produced by hyperglycaemia, by acting as scavengers of the superoxide radical. In addition, serotonin derivative concentration inside the cells and inside the mitochondria was increased in a time-dependent manner. Since recent studies support the assertion that mitochondrial dysfunctions related to oxidative damage are the major contributors to neurodegenerative diseases, these preliminary cell-based results identify a mitochondria-targeted antioxidant property of serotonin derivatives that could represent a novel therapeutic approach against the neuronal disorders and complications related to ROS.

Type
Full Papers
Copyright
Copyright © The Authors 2009

Hyperglycaemia is associated with the progression of diabetic neuropathy caused by an insufficiency of arterial blood flow due to hyperglycaemia-induced atherosclerosis(Reference Dyck and Thomas1, Reference Greene, Sima, Alberts, Rifkin and Porte2), suggesting that hyperglycaemia may also damage neuronal cells because of the increased oxidative stress associated with disease progression(Reference Holder, Holl and Bartz3, Reference Phelan, Ito and Loeken4). Mitochondria are a major source of intracellular reactive oxygen species (ROS) and are vulnerable to oxidative stress(Reference Szeto5); their dysfunction leads to cell death via apoptosis and/or necrosis, playing a crucial role in the majority of neurodegenerative diseases(Reference Phelan, Ito and Loeken4, Reference Szeto5). Synthetic and natural antioxidants are widely used against oxidative damage as food additives and for tissue protection; because of the potential carcinogenic activity of the synthetic molecules, natural antioxidants are desirable(Reference Fukushima, Sakata and Tagawa6). Many epidemiological and clinical studies have suggested that antioxidants play a preventive role in several oxidative stress-related diseases; however, many large-scale intervention trials have failed to demonstrate the beneficial effects of antioxidant vitamins(Reference Marchioli, Schweiger and Levantesi7). Recently, some independent laboratories have focused their attention on other dietary compounds, such as serotonin derivatives, which may exert significant antioxidant effects both in vitro and in vivo, concentrating on their anti-atherogenic properties.

N-(p-coumaroyl)serotonin (CS) and N-feruloylserotonin (FS), two serotonin conjugates, have been identified as the major phenolic constituents of defatted safflower seeds(Reference Koyama, Kuribayashi and Seki8, Reference Zhang, Nagatsu and Watanabe9), which are members of the indole hydroxycinnamic acid amides, with serotonin (5-HT), p-coumaric acid (p-ca) and ferulic acid (fa) representing components of their structures(Reference Ly, Kang and Choi10, Reference Piga, Naito and Kokura11). The hydroxycinnamic acid amides of serotonin, including CS and FS, are synthesised by the enzyme serotonin N-hydroxycinnamoyltransferase.

CS and FS are present in several wild-growing plants and their seeds, such as safflower (Carthamus tinctorius L.) used in herbal medicine in Eastern countries, and worldwide mainly for edible oil production(Reference Zhang, Nagatsu and Watanabe9, Reference Ly, Kang and Choi10), konnyaku (Amorphophallus konjac K. Koch) widely used as a traditional food all over Japan(Reference Niwa, Murakami and Ohtake12), Japanese barnyard millet (Echinochloa utilis Ohwi & Yabuno), widely used in Japan especially in cold districts because of its resistance to low temperatures and for its highly nutritious grains making it a good substitute for rice(Reference Watanabe13), Centaurea nigra L. and many species of the genus Centaurea, traditionally used for their antibacterial activity in the treatment of various foods(Reference Kumarasamy, Middleton and Reid14Reference Sarker, Savchenko and Whiting16), and maize bran and other grains used in a wide variety of ways, including home cooking, to increase the fibre content of various foods(Reference Choi, Lee and Kim17). Furthermore, their presence has also been detected in several vegetables(Reference Ly, Kang and Choi10) used widely around the world.

Some of their biological and chemical activities have already been reported; they possess antibacterial and free radical-scavenging activities(Reference Niwa, Murakami and Ohtake12Reference Kumarasamy, Middleton and Reid14, Reference Choi, Lee and Kim17), behave as antioxidants in plasma and on liver HDL-cholesterol and total cholesterol(Reference Cho, Lee and Kim18), suggested to increase proliferation of fibroblasts(Reference Kawashima, Hayashi and Takii19), inhibit the production of pro-inflammatory cytokines(Reference Kawashima, Hayashi and Takii19), inhibit LDL oxidation in apoE-deficient mice(Reference Koyama, Kuribayashi and Seki8), exert protection against the increase of ROS-dependent adhesion and migration molecules that represent the key events in the early stages of atherosclerogenesis(Reference Piga, Naito and Kokura11, Reference Piga, Naito and Kokura20), and show other benefits against cardiovascular risk in healthy human volunteers(Reference Koyama, Suzuki and Furukawa21). However, there are no reports ascribing a particular effect to these serotonin derivatives against high glucose-inducing neuronal damage, although several reported evidence of the involvement of high glucose on mitochondrial dysfunction and oxidative stress in neurodegenerative diseases(Reference Szeto5, Reference Ceriello22, Reference Lin and Beal23).

The PC12 cell line, derived from a rat pheochromocytoma of adrenal medulla, undergoes differentiation following treatment with nerve growth factor from a tumour cell (tumour-type) to a neuron-like cell phenotype (neuron-type)(Reference Greene24, Reference Greene, Connolly and Viscarello25). The neuron-type cell is known to express a variety of properties shared by neurons including the overall phenotype and has been successfully used over the years as a neuronal model to study neuronal functions(Reference Grohovaz, Zacchetti and Clementi26Reference Waki, Yano and Yoshimoto29).

The present study followed a cell-based approach to investigate the protective effect of CS and FS against damage associated with hyperglycaemia in PC12 cells.

Materials and methods

Cells

Undifferentiated PC12 cells (kindly provided by Dr Hirose, Department of Anaesthesiology, Kyoto Prefectural University of Medicine, Kyoto, Japan) were routinely maintained at 37°C in a humidified atmosphere of 95 % air and 5 % CO2 in Dulbecco's modified Eagle's medium–Ham's nutrient mixture F-12 (DMEM–F-12, 1:1; Invitrogen, Carlsbad, CA, USA), containing 17·5 mm-d-(+)-glucose, 10 % heat-inactivated fetal bovine serum and 5 % heat-inactivated horse serum. At 60 % of confluence, the cells were differentiated by the administration of nerve growth factor (100 ng/ml) to a DMEM–F-12 medium supplemented with 0·5 % fetal bovine serum and 0·5 % horse serum for 4 d, as previously described(Reference Koshimura, Tanaka and Murakami30). Differentiated PC12 cells without any treatment and growing in DMEM–F-12 medium containing sufficient d-(+)-glucose were used as control cells.

Cell treatment

Differentiated PC12 cells were treated with d-(+)-glucose at different concentrations (25, 50, 100 mmol/l) for specified periods (0, 24, 48, 72, 96 h) as well as with 50-mm-d-(+)-glucose (high glucose; HG) for 72 h, which represent the resulting 50 % lethal concentration (LC50), in the presence or absence of 10 μm-CS or -FS (kindly provided by Dr Koyama, Ajinomoto Co., Kawasaki, Japan), 10 μm-5-HT, -p-ca or -fa as the components of CS and FS structures or 40 μm-α-tocopherol which was used as a positive control (all from Sigma, St Louis, MO, USA). Glucose uptake was performed as previously described(Reference Zou, Wang and Shen31) using a fluorescent d-glucose analogue 2-[N-(7-nitrobenx-2-oxa-1,3-diazol-4-yl)amino]-2-deoxy-d-glucose (Invitrogen), which was used to monitor glucose uptake in living cells.

Cell viability

To evaluate cell viability, the 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide (Sigma) assay was performed as described previously(Reference Denizot and Lang32). The optical density of formazan was measured at 570 nm using a Multiskan Ascent plate reader (Bio-Rad Fluoromark, Melville, NY, USA).

Phosphatidylserine, which is confined to the inner membrane in normal healthy cells, becomes exposed at the outer plasma membrane of apoptotic cells(Reference Pigault, Follenius-Wund and Schmutz33). Exposure of phosphatidylserine is an early event, as it precedes cell membrane permeabilisation, cell shrinkage and nuclear condensation(Reference Pigault, Follenius-Wund and Schmutz33). Phosphatidylserine exposure was then analysed as described previously(Reference Pigault, Follenius-Wund and Schmutz33), and measured by the binding of annexin V-zFITC, according to the protocol outlined by the manufacturer of the Annexin V-FITC Apoptosis Detection kit (MBL, Nagoya, Japan). Cells that have lost membrane integrity allow propidium iodide (PI) to enter. Treated cells were also stained with PI (MBL, Nagoya, Japan), and analysed using a Cytomics FC500 Flow Cytometry System.

Caspase activity

Caspase activity was measured by assessing the cleavage of the Asp-Glu-Val-Asp peptide-conjugated p-nitroanilide (pNA)(Reference Casciola-Rosen, Nicholson and Chong34) (Caspase-3/CPP32 Colorimetric Protease Assay Kit; MBL, Nagoya, Japan), according to the manufacturer's protocol. Substrate cleavage, which resulted in the release of pNA (405 nm), was measured using a Multiskan Ascent plate reader (Bio-Rad). Absorbance units were converted to pmol pNA by extrapolating them on a standard curve generated using free pNA. Caspase activity was expressed as pmol pNA generated per mg protein (Bio-Rad protein assay).

Determination of intracellular reactive oxygen species

Intracellular ROS were detected using the fluorescent probe 2′,7′-dichlorofluorescin diacetate (Molecular Probes, Eugene, OR, USA) as described earlier(Reference Takahashi, Shibata and Niki35). Mitochondrial superoxide was detected using a MitoSOX™ mitochondrial superoxide indicator (Molecular Probes). Fluorescence was observed using the Cytomics FC500 Flow Cytometry System.

High-performance liquid chromatography analysis

A sample of cells was used for mitochondria extraction performed using a Mitochondria Isolation Kit (Pierce, Rockford, IL, USA) according to the manufacturer's protocol. Subsequently, CS and FS were extracted with methanol–PBS (4:1, v/v) and were measured by HPLC as described earlier(Reference Yoshida, Hayakawa and Habuchi36). In order to quantify the concentration, CS and FS levels were normalised by the total protein content (μmol/mg protein).

Data analysis

Statistical analysis was performed as described previously(Reference Patel, Crisostomo and Lahm37). All data of at least three separate experiments were expressed as mean values with their standard errors. Inter-group differences were assessed by one-way ANOVA followed by the post hoc Bonferroni test. In order to assess the individual effects of HG and the selected compounds, as well as any interactions existing between these two factors, a two-way ANOVA with post hoc comparison was performed. All statistical analyses were carried out using the GraphPad Prism 4 program (GraphPad Software, Inc., San Diego, CA, USA). Values of P < 0·05 were considered statistically significant.

Results

Effects of N-(p-coumaroyl)serotonin and N-feruloylserotonin on 50-mm-d-(+)-glucose-induced damage in PC12 rat pheochromocytoma cells

d-(+)-Glucose treatment decreased PC12 viability in a concentration- and time-dependent manner and the resulting 50 % lethal concentration (LC50) was 50 mmol/l at 72 h (Fig. 1(a)). The viability decreased to approximately 24 % (P < 0·05), 35 % (P < 0·01) and 44 % (P < 0·01) at 24, 48 and 72 h, respectively, at the concentration of 50 mmol/l. Simultaneous treatment of PC12 cells with CS or FS plus HG for 72 h (Fig. 1(b)) resulted in a significant inhibition of cell death (P < 0·001) in comparison with cells treated with α-tocopherol (P < 0·001), while treatment with 10 μm-5-HT, -p-ca or -fa resulted in a significant but less protection (P < 0·05). Cells were also incubated with annexin V-FITC and PI, and then subjected to flow cytometry analysis (Fig. 1(c)). The percentage of apoptotic cells (annexin V-FITC-positive and PI-negative cells) among the HG-treated cells was 14-fold higher than among control cells (from 2·7 % of the controls to 37·9 % of HG); CS and FS treatment was associated with a significant inhibition of apoptosis (P < 0·01).

Fig. 1 Effects of 10 μm-N-(p-coumaroyl)serotonin (CS) and 10 μm-N-feruloylserotonin (FS) on 50-mm-d-(+)-glucose (HG)-induced damage in PC12 rat pheochromocytoma cells. (a) Concentration- and time-dependent viability. (–○–), Control (cells without any HG treatment); (- -●- -), 25 mm-HG; (–□–), 50 mm-HG; (- -■- -), 100 mm-HG. Values are means, with their standard errors represented by vertical bars. Mean value was significantly different from that of the control treatment at the same time point: * P < 0·05, ** P < 0·01, *** P < 0·001. (b) Effect of the selected compounds on HG-inducing cell death. C, control treatment; 5-HT, 10 μm-serotonin; p-ca, 10 μm-p-coumaric acid; fa, 10 μm-ferulic acid; α-toc, 40 μm-α-tocopherol. Mean value was significantly different from that of the HG-alone treatment: * P < 0·05, *** P < 0·001. ††† Mean value was significantly different from that of the control treatment (P < 0·001). (c) Effect of CS and FS on HG-inducing apoptosis. (□), Living cells; (■), apoptotic cells; (▧), necrotic cells. ** Mean value was significantly different from that of the HG-alone treatment (P < 0·01). †† Mean value was significantly different from that of the control treatment (P < 0·01).

Effects of N-(p-coumaroyl)serotonin and N-feruloylserotonin on 50-mm-d-(+)-glucose-induced caspase activity in PC12 rat pheochromocytoma cells

The caspase activity was analysed to confirm the ability of CS and FS to protect against apoptotic cell death caused by this stressor. As shown in Fig. 2(a), treatment of PC12 cells with HG caused a significant but transient increase in the caspase activity from 6 to 48 h, being significant at 24 h (P < 0·01) and 48 h (P < 0·05). Caspase activity increased and decreased in a time-dependent manner and the resulting highest activity was approximately two-fold higher (34·4 pmol pNA/mg protein) than for control cells (16·3 pmol pNA/mg protein) at 24 h. Thus CS and FS protection against caspase activity increase was analysed at 24 h. Simultaneous treatment of PC12 cells with CS or FS plus HG for 24 h (Fig. 2(b)) resulted in a significant inhibition of caspase activity (P < 0·01), stronger than that exerted by α-tocopherol (P < 0·05).

Fig. 2 Effects of 10 μm-N-(p-coumaroyl)serotonin (CS) and 10 μm-N-feruloylserotonin (FS) on 50-mm-d-(+)-glucose (HG)-induced caspase-3 activity in PC12 cells. Caspase-3 activity was measured by the cleavage of the Asp-Glu-Val-Asp (DEVD) peptide-conjugated p-nitroanilide (pNA) and expressed per mg total protein content. (a) Effect of HG on caspase-3 activity. Values are means, with their standard errors represented by vertical bars. Mean value was significantly different from that at time 0: * P < 0·05, ** P < 0·01. (b) Effect of the selected compounds on HG-inducing caspase activity. C, control (cells without any treatment); 5-HT, 10 μm-serotonin; p-ca, 10 μm-p-coumaric acid; fa, 10 μm-ferulic acid; α-toc, 40 μm-α-tocopherol. Mean value was significantly different from that of the HG-alone treatment: * P < 0·05, ** P < 0·01. †† Mean value was significantly different from that of the control treatment (P < 0·01).

Effect of N-(p-coumaroyl)serotonin and N-feruloylserotonin on 50-mm-d-(+)-glucose-induced intracellular reactive oxygen species

To understand the underlying mechanisms of CS and FS protection against HG damage, we examined the ROS-scavenging activity of CS and FS. The HG-induced caspase activation on PC12 was preceded by a significant increase in the intracellular ROS levels (P < 0·01 at 6, 12, 24 h), as shown by the 2′,7′-dichlorofluorescin fluorescence (Fig. 3(a)). The peak of fluorescence was reached at 12 h, although this increase was significant from 6 h, and was significantly reduced by CS and FS (P < 0·01) (Fig. 3(b)). 40 μm-α-Tocopherol had a similar effect to 10 μm-CS and -FS, while treatment with 10 μm-p-ca or -fa resulted in a lower but still significant reduction of ROS fluorescence (P < 0·05) (Fig. 3(b)). A similar protocol was performed using a MitoSOX™ fluorescent probe, specific for mitochondrial superoxide. The four-fold increased fluorescence by HG at 6 h was significantly reduced by CS and FS (P < 0·01) (Fig. 3(c) and (d)); 40 μm-α-tocopherol resulted in a lower but still significant reduction of MitoSOX™ fluorescence (P < 0·05) (Fig. 3(c)).

Fig. 3 Effect of 10 μm-N-(p-coumaroyl)serotonin (CS) and 10 μm-N-feruloylserotonin (FS) on 50-mm-d-(+)-glucose (HG)-induced intracellular reactive oxygen species (ROS) in PC12 cells. (a) Time-dependent intracellular ROS assessed by the fluorescence intensity of 2′,7′-dichlorofluorescin (DCF) emission in control (- -○- -) and HG-treated (–●–) cells. Values are means, with their standard errors represented by vertical bars. ** Mean value was significantly different from that at time 0 (P < 0·01). (b) Effect of the selected compounds on HG-inducing intracellular ROS assessed by the fluorescence intensity of DCF emission. C, control (cells without any treatment); 5-HT, 10 μm-serotonin; p-ca, 10 μm-coumaric acid; fa, 10 μm-ferulic acid; α-toc, 40 μm-α-tocopherol. Mean value was significantly different from that of the HG-alone treatment: * P < 0·05, ** P < 0·01. †† Mean value was significantly different from that of the control treatment (P < 0·01). (c) Effect of the selected compounds on HG-inducing intracellular ROS assessed by the fluorescence intensity of MitoSOX™ emission. Mean value was significantly different from that of the HG-alone treatment: * P < 0·05, ** P < 0·01. †† Mean value was significantly different from that of the control treatment (P < 0·01). (d) Flow-cytometry images of MitoSOX™ fluorescence.

N-(p-coumaroyl)serotonin and N-feruloylserotonin concentration inside PC12 rat pheochromocytoma cells and mitochondria

Treatment with 20 μm-CS from 0 to 96 h resulted in a time-dependent increase of CS concentration in cells and in mitochondria, reaching significance after 24 h in cells (10·4 μmol CS/mg protein; P < 0·01), and in mitochondria (4·3 μmol CS/mg protein; P < 0·05) (Fig. 4(a)). A similar pattern was obtained for FS detection in cells (9·6 μmol FS/mg protein; P < 0·01) and in mitochondria (2·9 μmol FS/mg protein; P < 0·05) (Fig. 4(b)).

Fig. 4 N-(p-coumaroyl)serotonin (CS) (a) and N-feruloylserotonin (FS) (b) concentration inside PC12 whole cells (–●–) and mitochondria (- -○- -). CS and FS levels were normalised by the total protein content (μmol/mg protein). Values are means, with their standard errors represented by vertical bars. Mean value was significantly different from that at time 0: * P < 0·05, ** P < 0·01, *** P < 0·001.

Discussion

We previously reported that CS and FS, two serotonin conjugates, exerted their benefits against hyperglycaemic disorders and complications related to ROS(Reference Piga, Naito and Kokura11). Although increasing evidence suggests that CS and FS are protective against endothelial damage both in vitro and in vivo animals and human subjects(Reference Koyama, Kuribayashi and Seki8, Reference Piga, Naito and Kokura11, Reference Koyama, Suzuki and Furukawa21), to the best of our knowledge, cell-based studies on their action against neuronal damage have not been reported. Since mitochondrial dysfunction and oxidative stress are often correlated with hyperglycaemia(Reference Szeto5, Reference Ceriello22, Reference Lin and Beal23), we questioned whether CS and FS have the potential to safely modulate oxidative stress in a neuronal system of hyperglycaemia toxicity, acting as protective compounds as they do in vascular systems.

In our cell-based neuronal-like system of hyperglycaemia toxicity, we found that the simultaneous treatment of PC12 with HG plus CS or FS reduced HG-induced cell death. Since the literature on CS and FS is scarce and in order to quantify their antioxidant capacity, we compared the effects of CS and FS with those of α-tocopherol at a dietary relevant level (40 μmol/l). α-Tocopherol is able to protect neuronal and PC12 cells from cell damage induced by several stresses including high glucose(Reference Kumarasamy, Middleton and Reid14, Reference Kaliora, Dedoussis and Schmidt38, Reference Liu, Zubik and Collins39). Koyama et al. (Reference Koyama, Suzuki and Furukawa21) did not measure directly the human plasma concentration of CS and FS, but they observed a whole-blood serotonin increase in association with CS or FS intake, while Tanno et al. (Reference Tanno, Ichiyanagi and Ikeshiro40) measured a rapid absorption and relatively high blood concentrations of CS and FS in rats after oral administration. Although the present results are restricted to a cell-based approach, together with the evidence reported in the literature, it may be suggested that CS and FS are protective in our model and that levels necessary for this protection can be achieved through dietary means. We also compared the present results with the effect of 5-HT, p-ca or fa, which are the components of CS and FS structure, in order to show that the protection provided by FS and CS was greater than any component of their structure; CS and FS protection was higher than that of 5-HT, p-ca or fa alone in the experimental conditions used. Since 5-HT, p-ca and fa offer protection against cell death caused by stressors including glucose(Reference Kaliora, Dedoussis and Schmidt38, Reference Liu, Zubik and Collins39, Reference Galati, Sabzevari and Wilson41Reference Yogeeta, Raghavendran and Gnanapragasam44), the present results suggest that protection offered by CS and FS may be due to both 5-HT and p-ca or fa moieties acting together. CS and FS protection was further demonstrated by using annexin V-FITC and PI fluorescent probes, allowing us to discriminate between apoptotic and necrotic cell death, underlining the ability of CS and FS to protect against apoptosis, which resulted as being the type of cell death resultant from HG. This result suggests that CS and FS may act in one or more of the cascade of events leading to apoptosis.

In order to understand the protective mechanisms against cytotoxicity and the effect on the apoptotic process, we examined the effect of CS and FS on caspase activity and ROS production. Hyperglycaemia may damage neuronal cells by increasing oxidative stress associated with a progression of diabetic neuropathy(Reference Holder, Holl and Bartz3, Reference Phelan, Ito and Loeken4). Mitochondria are the major endogenous producers of ROS, and they have been implicated in the control of cell death(Reference Oliveira and Rego45). Mitochondria producing ROS could activate apoptotic cells death in two ways; through caspase-dependent and/or -independent pathways(Reference Oliveira and Rego45). Caspase-3 is required for the cleavage of the DNA fragmentation factor DFF, which has the nuclease activity responsible for DNA fragmentation during apoptosis(Reference Oliveira and Rego45). Mitochondria, on the other hand, after apoptotic insult release apoptotic-inducing factor into the cytosol, which translocates to the nucleus where it binds to the DNA and induces its fragmentation, independently of caspase activity(Reference Oliveira and Rego45). We tested the effect of CS and FS in comparison with the effects of α-tocopherol, 5-HT, p-ca and fa on HG-induced caspase activity, to evaluate their role in PC12 cell death. The mitochondrial ROS distribution was also determined to clarify and compare their ability to penetrate inside mitochondria, and their role against superoxide, which is one of the most damaging radicals produced by hyperglycaemia(Reference Ceriello46). The present results underline a role for caspase-3 in HG-inducing PC12 cell death; decreased activity of caspase-3 and cell loss due to increased cells death. Both CS and FS inhibited caspase activity, being more protective than α-tocopherol, which since none of the component structures affected caspase activity is probably associated with mitochondrial superoxide scavenging.

Although 2′,7′-dichlorofluorescin fluorescence was inhibited to different extents by each antioxidant used, only CS and FS possessed the ability to reduce the MitoSOX™ fluorescence –an ability that α-tocopherol also exerted with a similar fluorescence, being greater in treated than control cells. Since 2′,7′-dichlorofluorescin diacetate is not specific for superoxide, and does not penetrate selectively into mitochondria, this result means that superoxide is probably the chief radical produced by HG, and it is localised inside the mitochondria. All the antioxidants tested scavenge cytosolic ROS other than superoxide, while only CS and FS scavenge mitochondrial superoxide. α-Tocopherol, 5-HT, p-ca and fa activity against several ROS is already documented in the literature(Reference Kaliora, Dedoussis and Schmidt38, Reference Liu, Zubik and Collins39, Reference Galati, Sabzevari and Wilson41Reference Yogeeta, Raghavendran and Gnanapragasam44). The present results, therefore, suggest a more powerful and selective antioxidant activity for CS and FS against mitochondrial superoxide which could be explained by a greater ability to cross the mitochondrial membrane. In fact, all the isoforms of vitamin E are lipophilic and are retained in cell membranes, failing to achieve significant intracellular concentrations as well at the relevant sites of free radical generation(Reference Szeto5), while fa shows more pronounced mitigation of ROS in a combination with both ascorbic acid and vitamin E(Reference Yogeeta, Raghavendran and Gnanapragasam44). The benefits of p-ca under physiological conditions may be counteracted by its pro-oxidant activity(Reference Galati, Sabzevari and Wilson41, Reference Kojima and Takeuchi42). These different actions with respect to scavenging superoxide could also explain their respective capacities to prevent cell death.

Since MitoSOX™ results confirmed an early uptake of CS and FS into the mitochondria, we quantified the concentration of both compounds inside the PC12 cells and their mitochondria by HPLC. Treatment of PC12 cells with CS or FS revealed a time-dependent increase in CS or FS cell and mitochondrial concentrations, suggesting a potential role for CS and FS as protective against oxidative insult particularly because of their stability, which does not show a time-dependent modification, transformation or degradation.

The literature concerning CS and FS intake from the diet and impact in vivo is limited and almost always in relation to atherosclerotic CVD. Evidence supporting the involvement of environmental factors including diet in the incidence of CVD in the Far East is significantly less than in the West. Genetic reasons for this phenomenon may exist although the rate of this disease in ethnic immigrant populations in the West approaches that of the disease in native Caucasians(Reference Tunstall-Pedoe, Kuulasmaa and Amouyel47). Konnyaku and Japanese barnyard millet are both widely used as a traditional food all over Japan, the latter especially in cold districts because of its resistance to low temperatures and because its highly nutritious grains make it a good substitute for rice(Reference Niwa, Murakami and Ohtake12, Reference Watanabe13). Using a cell-based approach, the present study suggests a serotonin derivative-related mechanism against HG-inducing apoptosis in PC12 cells, due to antioxidant properties and ROS-scavenging abilities, in particular superoxide produced in mitochondria. Further studies are needed, especially in vivo, to elucidate other properties and the mechanism of action, which could better clarify the role of serotonin derivatives in this pathology. The present results suggest that these compounds could be taken into consideration to reduce risk against ROS-related neuronal dysfunctions.

Acknowledgements

The authors are employees of the Kyoto Prefectural University of Medicine and the work described in the present paper has been funded by a Grant-in-Aid for Scientific Research (15390178 TY) from the Ministry of Education, Culture, Sports, Science and Technology of Japan, from the Bio-oriented Technology Research Advancement Institution and from the Ministry of Agriculture, Forestry and Fisheries of Japan.

The authors are grateful to Professor Etsuo Niki, Professor Yoshiro Saito and Professor Yasukazu Yoshida, Human Stress Signal Research Centre, AIST Kansai, Japan, for their assistance on HPLC analysis and critical discussion of data.

All the authors designed the proposed study. R. P. conducted the experiments and drafted the paper. Y. N., S. K., O. H. and T. Y. provided helpful technical advice and support in all the experiments carried out, and also supervised the entire work.

The authors are employees of the Kyoto Prefectural University of Medicine. They declare no other conflicts of interest.

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Figure 0

Fig. 1 Effects of 10 μm-N-(p-coumaroyl)serotonin (CS) and 10 μm-N-feruloylserotonin (FS) on 50-mm-d-(+)-glucose (HG)-induced damage in PC12 rat pheochromocytoma cells. (a) Concentration- and time-dependent viability. (–○–), Control (cells without any HG treatment); (- -●- -), 25 mm-HG; (–□–), 50 mm-HG; (- -■- -), 100 mm-HG. Values are means, with their standard errors represented by vertical bars. Mean value was significantly different from that of the control treatment at the same time point: * P < 0·05, ** P < 0·01, *** P < 0·001. (b) Effect of the selected compounds on HG-inducing cell death. C, control treatment; 5-HT, 10 μm-serotonin; p-ca, 10 μm-p-coumaric acid; fa, 10 μm-ferulic acid; α-toc, 40 μm-α-tocopherol. Mean value was significantly different from that of the HG-alone treatment: * P < 0·05, *** P < 0·001. ††† Mean value was significantly different from that of the control treatment (P < 0·001). (c) Effect of CS and FS on HG-inducing apoptosis. (□), Living cells; (■), apoptotic cells; (▧), necrotic cells. ** Mean value was significantly different from that of the HG-alone treatment (P < 0·01). †† Mean value was significantly different from that of the control treatment (P < 0·01).

Figure 1

Fig. 2 Effects of 10 μm-N-(p-coumaroyl)serotonin (CS) and 10 μm-N-feruloylserotonin (FS) on 50-mm-d-(+)-glucose (HG)-induced caspase-3 activity in PC12 cells. Caspase-3 activity was measured by the cleavage of the Asp-Glu-Val-Asp (DEVD) peptide-conjugated p-nitroanilide (pNA) and expressed per mg total protein content. (a) Effect of HG on caspase-3 activity. Values are means, with their standard errors represented by vertical bars. Mean value was significantly different from that at time 0: * P < 0·05, ** P < 0·01. (b) Effect of the selected compounds on HG-inducing caspase activity. C, control (cells without any treatment); 5-HT, 10 μm-serotonin; p-ca, 10 μm-p-coumaric acid; fa, 10 μm-ferulic acid; α-toc, 40 μm-α-tocopherol. Mean value was significantly different from that of the HG-alone treatment: * P < 0·05, ** P < 0·01. †† Mean value was significantly different from that of the control treatment (P < 0·01).

Figure 2

Fig. 3 Effect of 10 μm-N-(p-coumaroyl)serotonin (CS) and 10 μm-N-feruloylserotonin (FS) on 50-mm-d-(+)-glucose (HG)-induced intracellular reactive oxygen species (ROS) in PC12 cells. (a) Time-dependent intracellular ROS assessed by the fluorescence intensity of 2′,7′-dichlorofluorescin (DCF) emission in control (- -○- -) and HG-treated (–●–) cells. Values are means, with their standard errors represented by vertical bars. ** Mean value was significantly different from that at time 0 (P < 0·01). (b) Effect of the selected compounds on HG-inducing intracellular ROS assessed by the fluorescence intensity of DCF emission. C, control (cells without any treatment); 5-HT, 10 μm-serotonin; p-ca, 10 μm-coumaric acid; fa, 10 μm-ferulic acid; α-toc, 40 μm-α-tocopherol. Mean value was significantly different from that of the HG-alone treatment: * P < 0·05, ** P < 0·01. †† Mean value was significantly different from that of the control treatment (P < 0·01). (c) Effect of the selected compounds on HG-inducing intracellular ROS assessed by the fluorescence intensity of MitoSOX™ emission. Mean value was significantly different from that of the HG-alone treatment: * P < 0·05, ** P < 0·01. †† Mean value was significantly different from that of the control treatment (P < 0·01). (d) Flow-cytometry images of MitoSOX™ fluorescence.

Figure 3

Fig. 4 N-(p-coumaroyl)serotonin (CS) (a) and N-feruloylserotonin (FS) (b) concentration inside PC12 whole cells (–●–) and mitochondria (- -○- -). CS and FS levels were normalised by the total protein content (μmol/mg protein). Values are means, with their standard errors represented by vertical bars. Mean value was significantly different from that at time 0: * P < 0·05, ** P < 0·01, *** P < 0·001.