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Cacao liquor procyanidin extract improves glucose tolerance by enhancing GLUT4 translocation and glucose uptake in skeletal muscle

Published online by Cambridge University Press:  31 May 2012

Yoko Yamashita
Affiliation:
Department of Agrobioscience, Graduate School of Agricultural Science, Kobe University, Nada-ku, Kobe 657-8501, Japan
Masaaki Okabe
Affiliation:
Food Science Research Labs, Meiji Co. Ltd, Sakado 350-0289, Japan
Midori Natsume
Affiliation:
Food Science Research Labs, Meiji Co. Ltd, Sakado 350-0289, Japan
Hitoshi Ashida*
Affiliation:
Department of Agrobioscience, Graduate School of Agricultural Science, Kobe University, Nada-ku, Kobe 657-8501, Japan
*
*Corresponding author: H. Ashida, Ph.D., fax + 81-78-803-5878, email ashida@kobe-u.ac.jp

Abstract

Hyperglycaemia and insulin resistance are associated with the increased risk of the metabolic syndrome and other severe health problems. The insulin-sensitive GLUT4 regulates glucose homoeostasis in skeletal muscle and adipose tissue. In this study, we investigated whether cacao liquor procyanidin (CLPr) extract, which contains epicatechin, catechin and other procyanidins, improves glucose tolerance by promoting GLUT4 translocation and enhances glucose uptake in muscle cells. Our results demonstrated that CLPr increased glucose uptake in a dose-dependent manner and promoted GLUT4 translocation to the plasma membrane of L6 myotubes. Oral administration of a single dose of CLPr suppressed the hyperglycaemic response after carbohydrate ingestion, which was accompanied by enhanced GLUT4 translocation in ICR mice. These effects of CLPr were independent of α-glucosidase inhibition in the small intestine. CLPr also promoted GLUT4 translocation in skeletal muscle of C57BL/6 mice fed a CLPr-supplemented diet for 7 d. These results indicate that CLPr is a beneficial food material for improvement of glucose tolerance by promoting GLUT4 translocation to the plasma membrane of skeletal muscle.

Type
Research Article
Copyright
Copyright © The Author(s) 2012. The online version of this article is published within an Open Access environment subject to the conditions of the Creative Commons Attribution-NonCommercial-ShareAlike licence <http://creativecommons.org/licenses/by-nc-sa/2.5/>. The written permission of Cambridge University Press must be obtained for commercial re-use.

Many countries are experiencing a rapid increase in the number of patients with diabetes mellitus, and type 2 diabetes mellitus in particular is a major health problem worldwide. The pathogenesis of type 2 diabetes mellitus involves progressive development of insulin resistance in peripheral tissues, combined with an insufficient pancreatic insulin secretion. It is also associated with inadequate suppression of glucagon secretion in response to ingested glucose, leading to overt hyperglycaemia(1). Insulin resistance, which is usually defined as an inadequate biological response of glucose metabolism to high insulin concentrations(Reference Hauner2), is associated with increased risk of CVD(Reference Alderman, Cohen and Madhavan3, 4) and diabetes(Reference Osei, Rhinesmith and Gaillard5). Although several studies have attempted to improve insulin sensitivity in subjects with impaired glucose tolerance by pharmacological approaches, as well as appropriate lifestyle and dietary modifications(Reference Dagogo-Jack, Egbuonu and Edeoga6Reference Distefano and Watanabe8), the success of these approaches has been limited in terms of normalisation of blood glucose levels, and novel approaches are still needed.

Epidemiological evidence and several clinical studies have demonstrated that foods rich in polyphenols, including fruits, vegetables, red wine, tea and cocoa, possess a wide range of health-promoting activities and may reduce the risk of CVD(Reference Ding, Hutfless and Ding9, Reference Deka and Vita10), diabetes(Reference Wolfram11, Reference Gin, Rigalleau and Caubet12) and hyperglycaemia(Reference Hanhineva, Törrönen and Bondia-Pons13, Reference Matsui, Tanaka and Tamura14), for example. It was also reported that some polyphenols can normalise blood glucose levels(Reference Hanhineva, Törrönen and Bondia-Pons13). Inhibition of α-glucosidase and other carbohydrate digestive enzymes is an established target of polyphenols for maintaining blood glucose levels. However, recent reports have focused on insulin-sensitive GLUT4 as a novel target of polyphenols(Reference Bryan, Govers and James15). GLUT4 is expressed in adipose tissue, skeletal muscle and cardiac muscle. Of these, skeletal muscle is one of a particularly therapeutic target for hyperglycaemia, because skeletal muscle accounts for approximately 80 % of insulin-stimulated glucose uptake in the postprandial state and plays a vital role in maintaining glucose homoeostasis(Reference Saltiel and Kahn16).

Translocation of GLUT4 from the intracellular pool to the plasma membrane in skeletal muscle is induced by insulin-dependent and insulin-independent mechanisms and is followed by glucose uptake and incorporation into the cells. Insulin promotes GLUT4 translocation via a phosphatidylinositol 3-kinase-dependent mechanism, whereas exercise and contraction promotes insulin-independent translocation of GLUT4 by activating AMP-activated protein kinase (AMPK)(Reference Hardie17). Resveratrol, a phytoalexin present in the skin of grapes and red wine, stimulates glucose uptake and translocation of GLUT4 in cultured L6 myotubes by activating both insulin- and AMPK-dependent signalling pathways(Reference Minakawa, Kawano and Miura18). However, we previously reported that (−)-epigallocatechin-3-gallate promotes GLUT4 translocation in skeletal muscle of rodents in vivo and in L6 myotubes in vitro by a mechanism that is at least partly independent of insulin(Reference Ueda, Nishiumi and Nagayasu19). (−)-Epigallocatechin-3-gallate was reported to increase AMPK phosphorylation(Reference Ahang, Li and Liang20), indicating that the AMPK-dependent signalling pathway at least partly contributes to (−)-epigallocatechin-3-gallate -stimulated GLUT4 translocation. Moreover, intake of green and black tea retained a decrease in the GLUT4 and insulin receptor expression levels of in high-fat diet-fed C57BL/6 mice(Reference Nishiumi, Bessyo and Kubo21, Reference Imada, Tanaka and Nishiumi22). These results indicate that polyphenols have potential to increase translocation and/or expression of GLUT4 in peripheral tissues, including skeletal muscle, which explains their prevention of hyperglycaemia and insulin resistance.

Cacao liquor procyanidin (CLPr), extracted from cacao liquor, an ingredient of chocolate and cocoa, is rich in polyphenols(Reference Crozier, Preston and Hurst23Reference Adamson, Lazarus and Mitchell25) such as monomeric epicatechin and catechin, and oligomeric procyanidins(Reference Urpi-Sarda, Monagas and Khan24). These polyphenols have potent antioxidant activities in vitro (Reference Gu, House and Wu26, Reference Hatano, Miyatake and Natsume27). Grassi et al. (Reference Grassi, Lippi and Necozione28Reference Grassi, Desideri and Necozione30) reported that the consumption of dark chocolate increased insulin sensitivity in healthy subjects(Reference Grassi, Lippi and Necozione28) and hypertensive patients(Reference Grassi, Necozione and Lippi29, Reference Grassi, Desideri and Necozione30). Tomaru et al. (Reference Tomaru, Takano and Osakabe31) reported that dietary supplementation with CLPr prevents the development of hyperglycaemia in db/db mice. However, the physiological and molecular mechanism by which CLPr improves glucose tolerance is not yet fully understood. Therefore, in the present study, we investigated whether CLPr promotes GLUT4 translocation and increases glucose uptake in skeletal muscle cells in vivo and in vitro.

Materials and methods

Materials

CLPr was prepared from cacao liquor as previously described(Reference Osakabe, Yamagishi and Sanbongi32, Reference Natsume, Osakabe and Yamagishi33). Polyphenol composition of CLPr was quantified by HPLC and liquid chromatography–MS, as detailed previously(Reference Natsume, Osakabe and Yamagishi33, Reference Yasuda, Natsume and Sasaki34). The amounts of individual procyanidins are represented as epicatechin equivalents. The total amount of polyphenol was measured by the Prussian Blue method(Reference Price and Butler35). The composition of polyphenols in CLPr is shown in Table 1. Glucose was measured using a commercially available kit (Labassay™ Glucose Wako kit, Wako Pure Chemical Industries, Ltd). The radiolabelled glucose analogue 2-[Reference Alderman, Cohen and Madhavan3H]deoxy-d-glucose was purchased from American Radiolabeled Chemicals Inc. Insulin concentrations were measured using an insulin assay kit from Shibayagi Co. Dulbecco's modified Eagle's medium, penicillin G and rat intestinal acetone powder were from Sigma–Aldrich. Fetal bovine serum and streptomycin were from BioWest S.A.S. and MP Biomedicals Inc., respectively. Bovine serum albumin (fatty acid and insulin free) and polyvinylidene difluoride membranes were from Nacalai Tesque Inc. and Pall Co., respectively. Anti-GLUT1, anti-GLUT4, anti-β-actin and horseradish peroxidase-conjugated anti-goat and anti-mouse IgG antibodies were purchased from Santa Cruz Biotechnology Inc. All other reagents used were of the highest grade available from commercial sources.

Table 1. Polyphenol composition of cacao liquor extract (CLPr)*

* The polyphenol composition was quantified by HPLC and liquid chromatography–MS, as previously described previously(Reference Natsume, Osakabe and Yamagishi33).

The amounts of procyanidins in the extract are given as epicatechin equivalents(Reference Yasuda, Natsume and Sasaki34).

The total amount of polyphenol was measured by the Prussian Blue method(Reference Price and Butler35).

Cell culture and treatment with cacao liquor procyanidin

L6 myoblasts (passage 27–37) were maintained in Dulbecco's modified Eagle's medium supplemented with 10 % (w/v) fetal bovine serum, penicillin G (100 units/ml), and streptomycin (100 µg/ml) at 37°C under a humidified atmosphere of 5 % CO2. The L6 myoblasts were seeded on twenty-four-well plates or 60-mm dishes and grown to a semi-confluent state. After 2 d, the medium was replaced with Dulbecco's modified Eagle's medium containing 2 % fetal bovine serum. The myoblasts were cultured for a further 5 d, and the medium was replaced every 2 d. Myotubes were incubated in serum-free Dulbecco's modified Eagle's medium containing 0·2 % (w/v) bovine serum albumin for 18 h, and then treated with CLPr solution or dimethylsulfoxide (DMSO) as a vehicle control. CLPr, which was prepared by dissolving 250 mg/ml CLPr in DMSO, was added to the cells at the indicated concentrations.

Measurement of glucose uptake activity

The differentiated L6 myotubes on twenty-four-well plates were incubated with 300 µl of Krebs-Ringer-HEPES buffer (50 mmol/l HEPES, pH 7·4, 137 mmol/l NaCl, 4·8 mmol/l KCl, 1·85 mmol/l CaCl2, and 1·3 mmol/l MgSO4) at 37°C and treated with CLPr (0·05–10 μg/ml) or insulin (100 nmol/l) for 15 min. Then, the cells were incubated with 6·5 mmol/l 2-[3H]deoxy-d-glucose (18 kBq/well) for a further 5 min. Next, the cells were washed five times with ice-cold Krebs-Ringer-HEPES buffer and solubilised in 0·05 mol/l NaOH. The radioactivity of 2-[3H]deoxy-d-glucose incorporated into the cells was measured by a liquid scintillation counter with a scintillation cocktail. Non-specific 2-[3H]deoxy-d-glucose uptake was determined by treating cells with 20 µmol/l cytochalasin B before adding CLPr.

Cytotoxicity

The cytotoxicity of CLPr was determined by crystalviolet staining, following the treatment of L6 myotubes on twenty-four-well plate with DMSO or CLPr (0·1–100 mg/ml) in 0·2 % (w/v) bovine serum albumin/minimum essential medium for 15 min. Then, the cell were fixed and stained with 2 % ethanol containing 0·2 % (w/v) Crystal Violet for 10 min. The wells were washed three times with tap water, and the stained cells were extracted with 50 % ethanol containing 0·5 % w/v SDS. The absorbance at 570 nm with a reference wavelength of 630 nm was measured using the Wallac 1420 ARVOsx.

Preparation of the plasma membrane and whole protein fractions

The plasma membrane fraction was prepared from CLPr-treated myotubes as previously described(Reference Nishiumi and Ashida36) to investigate whether CLPr stimulates GLUT4 translocation from intracellular storage vesicles to the plasma membrane. Briefly, myotubes were treated with CLPr (1–10 μg/ml), insulin (100 nmol/l) or DMSO as a vehicle control for 15 min, washed twice with ice-cold Krebs-ringer-HEPES buffer, homogenised in buffer A (50 mmol/l Tris, pH 8·0, 0·1 % (v/v) Nonidet P-40, 0·5 mmol/l dithiothreitol (DTT), protease inhibitors (1 mmol/l phenylmethylsulfonyl fluoride, 5 μg/ml leupeptin and 5 μg/ml aprotinin) and phosphatase inhibitors (10 mmol/l NaF and 1 mmol/l Na3VO4)) using a hand-held microtube homogeniser, and passed through a twenty-seven-gauge syringe needle five times. Part of the homogenate was mixed with radio immunoprecipitation assay (RIPA) buffer (10 mmol/l Tris, pH 8·0, 150 mmol/l sodium chloride, 0·5 % (w/v) sodium deoxycholate, 0·1 % (w/v) SDS, 1 % (v/v) Nonidet P-40 and 0·5 mmol/l DTT) containing the same protease and phosphatase inhibitors and incubated on ice for 60 min with occasional mixing. The supernatant obtained after centrifugation at 16 000 g for 20 min at 4°C was referred to as the cell lysate. The remainder of the homogenate was centrifuged at 900 g for 10 min at 4°C. The resulting pellet was suspended in buffer A and centrifuged under the same conditions. The precipitate was resuspended in buffer A containing 1 % (v/v) Nonidet P-40 and the same protease and phosphatase inhibitors, incubated on ice for 60 min with occasional mixing, and centrifuged at 16 000 g for 20 min at 4°C. The resulting supernatant was used as the plasma membrane.

Animals and administration of cacao liquor procyanidin

All animal experiments were approved by the Institutional Animal Care and Use Committee (Permission No. 21-07-02) and carried out according to the guidelines for animal experiments at Kobe University. Male ICR and C57BL/6 mice (4 weeks old) were obtained from Japan SLC Inc. and maintained in a temperature-controlled room (23 ± 2°C) with a 12 h light–12 h dark cycle (lights on at 09.00 hours). The ICR mice were acclimatised for 7 d with free access to a commercial standard mouse diet consisting of 76 % carbohydrate, 15 % protein and 9 % fat (3·850 kcal/g diet; Research Diets) and tap water. These ICR mice were used for the following oral carbohydrate loading test.

To examine the effects of consecutive administration of CLPr on GLUT4 translocation, male C57BL/6 mice (4 weeks old) were used after acclimatisation for 7 d with free access to a commercial chow and tap water. The mice were randomly divided into three groups of four mice and given a diet containing 0, 0·5 or 1 % (w/w) CLPr. After 7 d of feeding, the mice were killed under anesthesia induced by an intraperitoneal injection of sodium pentobarbital. Blood samples were collected after cardiac puncture and placed in heparinised microcentrifuge tubes to prepare plasma by centrifugation at 9600 g for 10 min at 4°C. The plasma samples were used to measure glucose level. The hindlimb soleus muscle was excised, chopped into small pieces and homogenised in 10 volumes of buffer A. The plasma membrane was prepared for Western blotting analysis as previously described(Reference Nishiumi and Ashida36).

Oral carbohydrate loading test

In Experiment 1, CLPr (50 or 250 mg/kg body weight) or water alone (5 ml/kg body weight) was orally administered to ICR mice after an 18 h fast. After the 60 min administration of CLPr, the mice in each group were orally given 1 g/kg body weight of soluble starch, maltose, sucrose or glucose. Tail vein blood samples were collected in heparinised tubes at 0 (before administration), 15, 30, 60 and 120 min after the carbohydrate load and centrifuged at 9600 g for 10 min at 4°C to prepare plasma.

In Experiment 2, mice were given an oral dose of CLPr in water (250 mg/kg body weight (C)) or water alone (5 ml/kg body weight (W)) after an 18 h fast. Then, the mice in each group were subdivided into two groups of four mice. One group was orally administered with glucose (1 g/kg body wt (G)), while the other received water alone (5 ml/kg body wt (W)). Thus, the mice used in Experiment 2 were divided into four groups designated CLPr-water, CLPr-glucose, water–water and water–glucose. The mice were killed 30 min after the glucose or water administration under anaesthesia induced by an intraperitoneal injection of sodium pentobarbital. Plasma samples were prepared from blood and used to measure the glucose and insulin levels. The plasma membrane of the soleus muscle was prepared and used for Western blotting(Reference Nishiumi and Ashida36).

Western blotting

Proteins in the plasma membrane and cell lysate fractions of myotubes and soleus muscles were separated by SDS-polyacrylamide gels and transferred to polyvinylidene difluoride membranes. After blocking with commercial Blocking one solution (Nacalai Tesque), the membranes were incubated with the specified primary antibodies overnight at 4°C, followed by the corresponding horseradish peroxidase-conjugated secondary antibody for 1 h at room temperature. The proteins bands were visualised using ImmunoStar® LD (Wako) and detected with a light-Capture II (ATTO Corp.).

Measurement of α-glucosidase activity in the small intestine

α-Glucosidase activity was measured in the small intestine of mice treated with 50 or 250 mg/kg body weight CLPr after an 18 h fast. Control mice were given water alone (5 ml/kg body weight). The mice were killed 60 min after CLPr or water administration under sodium pentobarbital anaesthesia, and the small intestine between the duodenum and the caecum was removed. The small intestine was opened longitudinally with scissors and washed twice with 1·15 % (w/v) ice-cold KCl solution. The intestinal mucosa was removed by scraping with a glass slide. The mucosal scrapings were homogenised with three volumes of 1·15 % KCl solution on ice. The homogenate was centrifuged at 1000 g for 10 min at 4°C, and the resultant supernatant was collected and used to measure maltase and sucrase–isomaltase activities. The reaction mixture consisted of 100 mmol/l maltose or sucrose as a substrate in 56 mmol/l maleate buffer (pH 6·0). The reaction was initiated by adding 100 or 250 µg protein/μl homogenate, respectively. After incubation at 37°C for 0, 20, 40, 60 and 120 min, the reaction was terminated by heating the mixture in boiling water for 10 min, and then placed on ice for 10 min. After centrifugation at 1000 g for 10 min, the glucose concentration in the supernatant was measured. After the linear regression of the glucose formation from the substrates was confirmed, the enzymatic activity was determined by the slope of the linear line and represented as nmol glucose released/min per mg protein.

To estimate the inhibitory effect of CLPr on α-glucosidase in vitro, the acetone powder of rat intestine (Sigma) was used as the enzyme source of α-glucosidase. A total of 50 mg of the acetone powder was homogenised in 10 ml of 56 mmol/l ice-cold maleate buffer (pH 6·0) and centrifuged at 10 000 g at 4°C for 30 min. The resulting supernatant was used as the crude enzyme solution. Then, 100 μl of the supernatant was pre-incubated with 900 μl of 56 mmol/l maleate buffer containing 0·01, 0·03, 0·06, 0·1 or 0·15 % CLPr (final concentration) at 37°C for 10 min. The reaction was initiated by adding 1·0 ml of 2 % (w/v) maltose or sucrose solution in maleate buffer. After incubation at 37°C for 0, 60 and 120 min, the reaction was terminated, and the glucose concentration in the reaction mixture was measured. The enzymatic activity was determined as described above.

Statistical analysis

Data are presented as means with their standard errors. The statistical significance of differences among groups was determined using the Dunnett multiple comparison test (Figs. 1 and 5), or the Tukey–Kramer multiple comparison test (Figs. 24 and Tables 2 and 3) with the level of significance set at P < 0·05.

Fig. 1. Effects of cacao liquor procyanidin (CLPr) on glucose uptake in L6 myotubes. Glucose uptake was measured in serum-starved L6 myotubes treated with 0·05–10 µg/ml CLPr for 15 min. Some cells were treated with DMSO or 100 nmol/l insulin as negative and positive controls, respectively. Values are means, with standard errors represented by vertical bars. * Mean value was significantly different from that of the control group (P < 0·05; Dunnett's test).

Fig. 2. Effects of cacao liquor procyanidin (CLPr) on GLUT4 translocation in L6 myotubes. Serum-starved L6 myotubes were treated with 1, 5 or 10 µg/ ml CLPr for 15 min, or with dimethylsulfoxide (DMSO) or 100 nmol/l insulin as negative and positive controls, respectively. The abundance of GLUT4 and GLUT1 protein in the plasma membrane of L6 myotubes (A) and GLUT4 and β-actin proteins in cell lysate (B) was determined by Western blotting. Each panel shows representative data from triplicate experiments. The density of each band was analysed and normalised to that of β-actin for the cell lysate or GLUT1 for the plasma membrane. Values are means, with standard errors represented by vertical bars (n 3).a,b,c Mean values with unlike letters were significantly different (P < 0·05; Tukey–Kramer multiple comparison test).

Fig. 3. Effects of cacao liquor procyanidin (CLPr) on GLUT4 translocation in skeletal muscle and plasma glucose and insulin levels in mice following a glucose load. CLPr (250 mg/kg body weight; C) or water alone (5 ml/kg body weight; W) were orally administered to ICR mice. Mice in each group were then subdivided into two groups and given glucose (1 g/kg body weight; G) or water (5 ml/kg body weight; W). CW, CLPr-water; CG, CLPr-glucose; WW, water–water; WG, water–glucose. Skeletal muscle tissue (soleus) was removed 30 min after the glucose load. The abundance of GLUT4 and GLUT1 proteins in the plasma membrane of the muscle (A) and GLUT4 and β-actin proteins in the tissue lysate (B) was determined by Western blotting. Each panel shows representative data from four mice. The density of each band was analysed and normalised to that of β-actin for the tissue lysate or GLUT1 for the plasma membrane. (C, D) Plasma glucose (C) and insulin (D) levels. Values are means, with standard errors represented by vertical bars (n 4).a,b Mean values with unlike letters were significantly different (P < 0·05; Tukey–Kramer multiple comparison test).

Fig. 4. Effects of 7 d of cacao liquor procyanidin (CLPr) administration on GLUT4 translocation in skeletal muscle and plasma glucose level. C57BL/6 mice were given a diet containing 0, 0.5 or 1 % (w/w) CLPr for 7-d, after which skeletal muscle was dissected. The abundance of GLUT4 and GLUT1 proteins in the plasma membrane of skeletal muscle (A) and GLUT4 and β-actin proteins in the tissue lysate (B) was determined by Western blotting. Each panel shows representative data from four mice. The density of each band was analysed and normalised to that of β-actin for the tissue lysate or GLUT1 for the plasma membrane. (C) Plasma glucose levels. Values are means, with standard errors represented by vertical bars (n 4).a,b Mean values with unlike letters were significantly different (P < 0·05; Tukey–Kramer multiple comparison test).

Fig. 5. Effects of cacao liquor procyanidin (CLPr) on the plasma glucose response to an oral carbohydrate load. ICR mice were treated with 50 (■) or 250 (▲) mg/kg body weight CLPr or water (5 ml/kg body weight; (•)). At 60 min after CLPr administration, the mice in each group were then given an oral load (1 g/kg body weight) of glucose (A), soluble starch (B), maltose (C) or sucrose (D). Plasma glucose levels were measured at 0, 15, 30, 60 and 120 min after the carbohydrate load. Values are means, with standard errors represented by vertical bars, of triplicate independent experiments consisting of three mice per group. *Mean value was significantly different from the corresponding control group (P < 0·05; Dunnett's test).

Table 2. Area under the curve (AUC; mmol/l×120 min×10−2) of plasma glucose level* (Mean values with their standard errors of triplicate independent experiments consisting of three mice per group)

CLPr, cacao liquor procyanidin.

* AUC were calculated using the trapezoidal rule from the data presented in Fig. 5.

a,bMean values within a row with unlike superscript letters with significantly different (P < 0·05; Tukey–Kramer multiple comparison test).

Table 3. Effects of cacao liquor procyanidin (CLPr) on α-glucosidase in vivo and in vitro * (Mean values with their standard errors; n 3)

* α-Glucosidase activity was measured in the jejunum of CLPr-treated mice (A) or in the CLPr-treated homogenate of rat intestinal acetone powder (B).

a,b,cMean values within a row with unlike superscript letters were significantly different (P<0·05; Tukey–Kramer multiple comparison test).

Results

Effects of cacao liquor procyanidin on glucose uptake and GLUT4 translocation in L6 myotubes

We first investigated the effects of CLPr on glucose uptake in L6 myotubes, since CLPr contains polyphenols, such as catechins and epicatechin (Table 1), which are known to modulate glucose uptake in L6 myotubes(Reference Ueda, Nishiumi and Nagayasu19). When L6 myotubes were treated with 100 nmol/l insulin for 15 min, glucose uptake increased by approximately 1·4-fold compared with the DMSO-treated negative control (Fig. 1). In the absence of insulin, CLPr increased glucose uptake in a dose-dependent manner except for 10 µg/ml. The maximum effect was observed at a CLPr dose of 5 µg/ml, which elicited a response similar to 100 nmol/l insulin. Therefore, the following experiments were carried out using 1, 5 and 10 µg/ml CLPr.

As would be expected, 100 nmol/l insulin significantly (P = 0·011) enhanced GLUT4 translocation in L6 myotubes from the intracellular storage vesicles to the plasma membrane as compared with DMSO-treated control cells (Fig. 2(A)). In the absence of insulin, 5 and 10 µg/ml CLPr significantly (P = 0·023 and P = 0·043, respectively) stimulated GLUT4 translocation to the plasma membrane. In contrast, the abundance of GLUT1 in the plasma membrane was unchanged. Moreover, CLPr did not affect the expression of GLUT4 in the cell lysate (Fig. 2(B)). These results indicate that CLPr stimulates GLUT4 translocation to the plasma membrane, and thus enhances glucose uptake capacity in muscle cells. In addition, CLPr did not show any cytotoxic effects by 100 µg/ml (data not shown).

Effect of a single oral administration of cacao liquor procyanidin on GLUT4 translocation and plasma glucose and insulin levels

Next, we investigated the effect of single oral administration of CLPr on GLUT4 translocation in the soleus muscle of ICR mice after a glucose load. As shown in Fig. 3(A), GLUT4 translocation in the water–glucose group was increased by approximately 1·4-fold compared with the water–water group. Interestingly, CLPr alone (CLPr-water group) stimulated GLUT4 translocation without a glucose load; GLUT4 translocation in the CLPr-water group was approximately 2·9-fold higher than that in the water–water group. Moreover, CLPr showed additive effects with glucose because GLUT4 translocation in the CLPr-glucose group was approximately 3·9-fold higher when compared with the water–water group. In contrast, CLPr did not affect the plasma membrane expression of GLUT1 (Fig. 3(A)) or tissue lysate GLUT4 expression (Fig. 3(B)).

In the same experiment, the plasma glucose level in the water–glucose group was significantly higher than that in the other groups (Fig. 3(C)). This indicates that pre-administration of CLPr suppressed the acute elevation in plasma glucose, with levels similar to that in the control group. Similar results were observed for plasma insulin levels as CLPr suppressed hyperinsulinaemia induced by the glucose load (Fig. 3(D)). Taken together, these results indicate that pre-administration of CLPr inhibited the hyperglycaemic and hyperinsulinaemic responses to a glucose load by promoting GLUT4 translocation to the plasma membrane of skeletal muscle.

Effects of consecutive administration of cacao liquor procyanidin on GLUT4 translocation and plasma glucose levels

GLUT4 translocation induced by CLPr was also examined in the skeletal muscle of mice treated with 0·5 or 1 % CLPr for 7 d. Dietary supplementation of CLPr did not affect food or water intake during the experimental period (data not shown). The final body weight of mice was also not affected by CLPr, being 21·1 (se 0·22) g, 21·3 (se 0·26) g and 20·7 (se 0·75) g in mice fed 0, 0·5 and 1 % CLPr, respectively. However, CLPr, particularly at a dose of 0·5 %, significantly enhanced GLUT4 translocation to the plasma membrane of skeletal muscle (Fig. 4(A)) without affecting plasma glucose levels (Fig. 4(C)). The expression of GLUT1 in the plasma membrane (Fig. 4(A)) and GLUT4 in the tissue lysate (Fig. 4(B)) was unchanged.

Effects of cacao liquor procyanidin on plasma glucose response to oral ingestion of carbohydrates

Fig. 5 shows the effect of oral administration of CLPr on the plasma glucose response to an oral load of soluble starch, maltose, sucrose or glucose. Plasma glucose levels in the control group (carbohydrate alone) increased in response to oral carbohydrate loading, reaching a peak at 15 min (soluble starch, maltose and sucrose) or 30 min (glucose), and then decreased with time. Following the glucose load, 250 mg/kg body weight CLPr significantly suppressed the transient increases in plasma glucose levels at 15 and 30 min (P < 0·05; Fig. 5(A)). The area under the curve of the plasma glucose levels showed similar results (Table 2), and was significantly reduced by 250 mg/kg body weight CLPr. CLPr dose-dependently suppressed the acute elevations in the plasma glucose levels after the soluble starch and maltose loads (P < 0·05; Fig. 5(B, C) and Table 2). On the other hand, CLPr tended to decrease the plasma glucose levels in sucrose-loaded mice (Fig. 5(D) and Table 2), although not significantly.

Effects of cacao liquor procyanidin on intestinal α-glucosidase activity

Oligomeric procyanidins from grape seed were reported to inhibit the enzymatic activity of intestinal α-glucosidases, including maltase and sucrase in vitro (Reference Schäfer and Högger37). Therefore, it is possible that a similar effect may be responsible for the decreases in postprandial blood glucose levels as described earlier. Therefore, we measured the inhibitory effects of CLPr on α-glucosidase activity in vivo and in vitro (Table 3). These experiments revealed that CLPr did not inhibit maltase or sucrose–isomaltase activities in vivo; although it did inhibit these enzymes in a dose-dependent manner in vitro (P < 0·05).

Discussion

Diabetes mellitus is characterised by chronic hyperglycaemia, which is involved in the development of obesity, CVD and hypertension(1Reference Alderman, Cohen and Madhavan3). Controlling the postprandial blood glucose excursions can prevent hyperglycaemia and improve insulin resistance(1, Reference Alderman, Cohen and Madhavan3). As a strategy for preventing and treating hyperglycaemia, we focused on GLUT, which play important roles in glucose homoeostasis by regulating cellular glucose uptake. GLUT4 is a major GLUT expressed in skeletal and cardiac muscle, and in adipose tissue specifically GLUT4 is responsible for the uptake of large amounts of glucose into cells following its translocation from intracellular storage vesicles to the plasma membrane in response to insulin stimulation and muscle contraction(Reference Huang and Czech38). In skeletal muscle, stimulation of glucose uptake is mostly attributed to increased translocation and redistribution of the GLUT4 to the plasma membrane(Reference Hauner2, Reference Huang and Czech38). In the present study, we showed that CLPr reduces postprandial glucose tolerance by stimulating GLUT4 translocation to the plasma membrane in cultured L6 myotubes in vitro (Figs. 1 and 2) and in murine skeletal muscle in vivo (Figs. 3 and 4). Moreover, CLPr prevented postprandial glucose tolerance following a carbohydrate load (Fig. 5) without inhibiting small intestinal α-glucosidase (Table 3). To our knowledge, this is the first report showing that CLPr promotes GLUT4 translocation in skeletal muscle, although a previous report showed that CLPr prevented the development of hyperglycaemia in db/db mice(Reference Tomaru, Takano and Osakabe31). Since GLUT4 is a key molecule involved in regulating glucose levels, CLPr is an attractive and beneficial food material for preventing hyperglycaemia.

The most important finding in this study was that CLPr promoted the translocation of GLUT4 in the absence of insulin in L6 myotubes and in skeletal muscle in mice. Moreover, we detected an additive effect of CLPr and glucose on GLUT4 translocation in vivo. These findings indicate that the molecular effects of CLPr are independent of insulin. The CLPr used in this study contained 4·28 % catechins, 6·12 % epicatechin and 7·64 % procyanidins (dimer to tetramer). These compounds probably contribute to the enhanced GLUT4 translocation because catechins and procyanidins were previously reported to suppress hyperglycaemia(Reference Pinent, Blay and Bladé39Reference Montagut, Onnockx and Vaqué41). In fact, we previously reported that catechins, particularly (−)-epigallocatechin-3-gallate, increased glucose uptake and enhanced GLUT4 translocation in L6 myotubes and in the skeletal muscle of rodents in vivo and ex vivo (Reference Ueda, Nishiumi and Nagayasu19). In 3T3-L1 cells, non-gallate-type catechins increased glucose uptake and GLUT4 translocation, whereas gallate-type catechins inhibited insulin-stimulated glucose uptake(Reference Ueda, Furuyashiki and Yamada42). Similarly, the intake of green and black tea increased GLUT4 translocation in skeletal muscle and maintained GLUT4 and insulin receptor expression in high-fat diet-fed C57BL/6 mice(Reference Alderman, Cohen and Madhavan3, Reference Nishiumi, Bessyo and Kubo21, Reference Imada, Tanaka and Nishiumi22). Although the effects of epicatechin and catechin on glucose uptake were weaker than those of other catechins in L6 myotubes(Reference Ueda, Nishiumi and Nagayasu19), a recent report demonstrated that epicatechin treatment conferred diabetic mice with a healthier and longer lifespan, and also improved skeletal muscle stress output and AMPKα activity in skeletal muscle(Reference Si, Fu and Babu40). Regarding procyanidins, it was reported that grape-seed procyanidin extract prevented the development of hyperglycaemia in streptozotocin-induced diabetic rats and high-fructose diet-induced insulin resistance rat(Reference Pinent, Blay and Bladé39, Reference Meeprom, Sompong and Suwannaphet43). Similarly, black soyabean seed extract, which also contains abundant procyanidins, also suppressed hyperglycaemia and obesity in high-fat diet-fed C57BL/6 mice(Reference Kanamoto, Yamashita and Nanba44). In vitro experiments revealed that grape-seed procyanidin extract also stimulated glucose uptake in 3T3-L1 adipocytes and L6E9 myotubes(Reference Pinent, Blay and Bladé39, Reference Montagut, Onnockx and Vaqué41). In 3T3-L1 adipocytes, the molecular mechanisms seemed to involve phosphorylation of the insulin receptor and phosphorylation of downstream signalling components, including Akt, p44/42 and p38 mitogen-activated protein kinase(Reference Pinent, Blay and Bladé39, Reference Montagut, Onnockx and Vaqué41). However, the molecular mechanisms by which procyanidins promote GLUT4 translocation are still unclear, because the cellular machinery controlling its translocation in muscle cells differs from that in adipose cells(Reference Bryan, Govers and James15, Reference Stöckli, Fazakerley and Coster45, Reference Rowland, Fazakerley and James46). Indeed, gallate-type catechins elicited different effects on glucose uptake between L6 myotubes and 3T3-L1 adipocytes(Reference Ueda, Nishiumi and Nagayasu19, Reference Ueda, Furuyashiki and Yamada42), and GLUT4 translocation increased in skeletal muscle but decreased in adipose tissue of rats fed green tea(Reference Ashida, Furuyashiki and Nagayasu47), Moreover, the composition of procyanidins differs between plants, suggesting that the functions of the procyanidin-rich plant extracts will differ. Regarding the bioavailability of procyanidins, several in vivo and in vitro studies are reported. For example, catechins and procyanidin dimers are detected in human plasma after ingestion of cocoa(Reference Holt, Lazarus and Sullards48, Reference Tomas-Barberan, Cienfuegos-Jovellanos and Marín49); free form of procyanidin dimers and trimers were detected in rat plasma after oral intake of a grape seed extract(Reference Serra, Macià and Romero50); and procyanidin dimers, trimers and tetramers were transported across Caco-2 cells(Reference Ou, Percival and Zou51). Further studies are needed to clarify the bioavailability and molecular mechanisms underlying the effects of CLPr in muscle cells.

CLPr prevented the transient increase in plasma glucose levels after a carbohydrate load. This preventive effect was observed not only for glucose loading but also for soluble starch and maltose loading. This result suggests that inhibition of α-glucosidase is involved in the preventive effects of CLPr on hyperglycaemia in vivo. Inhibition of intestinal α-glucosidase activity is a well-documented mechanism for the prevention of hyperglycaemia. However, our results clearly showed that CLPr did not inhibit intestinal α-glucosidase activity in vivo, even though it did inhibit the enzyme in vitro. Many reports have shown that certain polyphenols, including anthocyanins, catechins, quercetin and luteolin, can inhibit intestinal α-glucosidase activity in vitro (Reference Matsui, Ebuchi and Kobayashi52Reference Kim, Kwon and Son56). It was also reported that rutin inhibited α-glucosidase activity in vivo and in vitro (Reference Fontana, Cazarolli and Lavado53). Meanwhile, Schäfer & Högger(Reference Schäfer and Högger37) demonstrated that the inhibitory effects of oligomeric procyanidins on α-glucosidase activity were dependent on their molecular weight as tetrameric and hexameric procyanidins were more potent inhibitors than dimeric and trimeric procyanidins in vitro. However, we previously reported that long-term intake of green or black tea suppressed hyperglycaemia by modulating the expression and translocation of GLUT4 without inhibition of α-glucosidase activity(Reference Nishiumi, Bessyo and Kubo21). Taken together, these findings indicate that polyphenols have a potential to prevent hyperglycaemia by inhibiting α-glucosidase, although the evidence in vivo is less convincing. Our present findings provide strong evidence to support that CLPr improves glucose tolerance mainly by enhancing GLUT4 translocation and glucose uptake in skeletal muscle.

In conclusion, the results of this study indicate that CLPr enhances GLUT4 translocation in muscle cells in vitro and in vivo. GLUT4 translocation to the plasma membrane will facilitate glucose uptake and improve postprandial glucose tolerance. Therefore, CLPr offers a beneficial food for the prevention of hyperglycaemia and potentially diabetes mellitus.

Acknowledgements

This work was supported in part by Special Coordination Funds for Promoting Science and Technology and the Creation of Innovation Centers for Advanced Interdisciplinary Research Areas (Innovative Bioproduction Kobe) from MEXT, Japan. All authors approved the submission of the manuscript and contributed as follows. Y. Y. carried out experiments, statistical analysis and wrote the manuscript; M. O. prepared the CLPr extract and proof read the manuscript; M. N. analysed the polyphenol composition of the extract and proof read the manuscript; and H. A. conducted the experimental design, wrote and proof read the manuscript. All authors read and approved the final manuscript. There is no conflict of interest associated with the present study.

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Figure 0

Table 1. Polyphenol composition of cacao liquor extract (CLPr)*

Figure 1

Fig. 1. Effects of cacao liquor procyanidin (CLPr) on glucose uptake in L6 myotubes. Glucose uptake was measured in serum-starved L6 myotubes treated with 0·05–10 µg/ml CLPr for 15 min. Some cells were treated with DMSO or 100 nmol/l insulin as negative and positive controls, respectively. Values are means, with standard errors represented by vertical bars. * Mean value was significantly different from that of the control group (P < 0·05; Dunnett's test).

Figure 2

Fig. 2. Effects of cacao liquor procyanidin (CLPr) on GLUT4 translocation in L6 myotubes. Serum-starved L6 myotubes were treated with 1, 5 or 10 µg/ ml CLPr for 15 min, or with dimethylsulfoxide (DMSO) or 100 nmol/l insulin as negative and positive controls, respectively. The abundance of GLUT4 and GLUT1 protein in the plasma membrane of L6 myotubes (A) and GLUT4 and β-actin proteins in cell lysate (B) was determined by Western blotting. Each panel shows representative data from triplicate experiments. The density of each band was analysed and normalised to that of β-actin for the cell lysate or GLUT1 for the plasma membrane. Values are means, with standard errors represented by vertical bars (n 3).a,b,c Mean values with unlike letters were significantly different (P < 0·05; Tukey–Kramer multiple comparison test).

Figure 3

Fig. 3. Effects of cacao liquor procyanidin (CLPr) on GLUT4 translocation in skeletal muscle and plasma glucose and insulin levels in mice following a glucose load. CLPr (250 mg/kg body weight; C) or water alone (5 ml/kg body weight; W) were orally administered to ICR mice. Mice in each group were then subdivided into two groups and given glucose (1 g/kg body weight; G) or water (5 ml/kg body weight; W). CW, CLPr-water; CG, CLPr-glucose; WW, water–water; WG, water–glucose. Skeletal muscle tissue (soleus) was removed 30 min after the glucose load. The abundance of GLUT4 and GLUT1 proteins in the plasma membrane of the muscle (A) and GLUT4 and β-actin proteins in the tissue lysate (B) was determined by Western blotting. Each panel shows representative data from four mice. The density of each band was analysed and normalised to that of β-actin for the tissue lysate or GLUT1 for the plasma membrane. (C, D) Plasma glucose (C) and insulin (D) levels. Values are means, with standard errors represented by vertical bars (n 4).a,b Mean values with unlike letters were significantly different (P < 0·05; Tukey–Kramer multiple comparison test).

Figure 4

Fig. 4. Effects of 7 d of cacao liquor procyanidin (CLPr) administration on GLUT4 translocation in skeletal muscle and plasma glucose level. C57BL/6 mice were given a diet containing 0, 0.5 or 1 % (w/w) CLPr for 7-d, after which skeletal muscle was dissected. The abundance of GLUT4 and GLUT1 proteins in the plasma membrane of skeletal muscle (A) and GLUT4 and β-actin proteins in the tissue lysate (B) was determined by Western blotting. Each panel shows representative data from four mice. The density of each band was analysed and normalised to that of β-actin for the tissue lysate or GLUT1 for the plasma membrane. (C) Plasma glucose levels. Values are means, with standard errors represented by vertical bars (n 4).a,b Mean values with unlike letters were significantly different (P < 0·05; Tukey–Kramer multiple comparison test).

Figure 5

Fig. 5. Effects of cacao liquor procyanidin (CLPr) on the plasma glucose response to an oral carbohydrate load. ICR mice were treated with 50 (■) or 250 (▲) mg/kg body weight CLPr or water (5 ml/kg body weight; (•)). At 60 min after CLPr administration, the mice in each group were then given an oral load (1 g/kg body weight) of glucose (A), soluble starch (B), maltose (C) or sucrose (D). Plasma glucose levels were measured at 0, 15, 30, 60 and 120 min after the carbohydrate load. Values are means, with standard errors represented by vertical bars, of triplicate independent experiments consisting of three mice per group. *Mean value was significantly different from the corresponding control group (P < 0·05; Dunnett's test).

Figure 6

Table 2. Area under the curve (AUC; mmol/l×120 min×10−2) of plasma glucose level* (Mean values with their standard errors of triplicate independent experiments consisting of three mice per group)

Figure 7

Table 3. Effects of cacao liquor procyanidin (CLPr) on α-glucosidase in vivo and in vitro* (Mean values with their standard errors; n 3)