NS seeds were obtained from a local market in Mymensingh, Bangladesh. The extraction of NS seeds was performed as previously described (27). Briefly, the black seeds were washed with running tap water, air-dried and ground to powder form (0.2–0.3 mm particle size, to ensure homogeneity). A total of 800 g powdered seeds were extracted in a Soxhlet apparatus with petroleum ether. The extract obtained was evaporated to a viscous liquid at 40°C under reduced pressure (yield of 300 ml, 310.7 g and 39.2%). Gas chromatographic analysis of the final extract failed to identify significant amounts of n-hexane and n-heptane (0.1%), which are the major indicators for this distillate.

All experimental protocols employed herein were approved by the Committee on the Care of Laboratory Animal Resources of Chonbuk National University and were conducted in accordance with the Guide for the Care and Use of Laboratory Animals published by the US National Institutes of Health (Bethesda, MA, USA; NIH Publication no. 85–23, revised 1996). A total of forty male Sprague-Dawley rats (220–250 g, Samtako Bio Korea Co., Ltd., Daejeon, Korea) were used for all experiments. Animals were housed in cages maintained at 23±2°C with 50±5% humidity and subjected to a 12-h light/dark cycle. Food and water was available ad libitum prior to exercise. The NS extract was freshly dissolved in either distilled water and orally administered using a gavage with a dose of 2 g/kg/day. In addition, NS extract was administered on the 21st day, 1 h prior to the initiation of swimming exercise. Distilled water was administered for control group.

A pool for exhaustive swimming was designed especially for rats. The system consisted of a glass chamber (70 cm in height, 60 cm in length and 90 cm in width) filled with water to a height of 55 cm. The pool was equipped with a heating system and an air pumping system. To prevent floating during swimming, water bubbles were produced by tubes connected to the air pumping system. The temperature of the water within the glass chamber was maintained at 36±1°C via a thermostatically controlled heater located at the base of the chamber. The rats were individually applied to forced-swimming until exhaustion, which was defined as failure to rise to the surface of the water to breathe for 7 sec (28).

Blood was collected from the tail vein just before swimming and from the caudal vena cava following swimming. A Nova Stat Profile^® pHOx Ultra Analyzer system (Nova Biomedical, Waltham, MA, USA) was used to measure pH and to quantify levels of partial pressure of carbon dioxide (pCO₂₎, the partial pressure of oxygen (pO₂) and oxygen saturation (O_2sat). In addition, the concentrations of glucose, lactate and hemoglobin (Hb) were measured, along with hematocrit (Hct). Serum was immediately separated by centrifugation at 1,500 × g for 10 min following swimming and stored at −80°C until biochemical analysis. A Hitachi 7020 system (Hitachi Corporation, Tokyo, Japan) was used for analyses of total protein (TP), albumin, lactic dehydrogenase (LDH) and creatine kinase (CK) levels.

The liver and g. muscle were cut, weighed and homogenized in cold perchloric acid. The homogenate was centrifuged for 15 min at 15,000 × g at 4°C. The supernatant was carefully decanted. A standard glycogen (Sigma; St.Louis, MO, USA) and tissue extract were mixed with iodine-potassium iodide reagent for binding iodine to glycogen. The mixtures were measured by the SpectraMax M3 ELISA reader (Molecular Devices, LLC, Sunnyvale, CA, USA) at 460 nm wavelength.

Levels of malondialdehyde (MDA) in serum, liver and g. muscle were measured with an OXI-TEK TBARS assay kit (Enzo Life Sciences Inc., Farmingdale, NY, USA). Reaction products were quantitated by measuring the absorbance at 532 nm according to the manufacturer's protocol. The levels of superoxide dismutase (SOD) in the serum, liver and g. muscle were quantitated using a SOD activity kit (cat. no. ADI-900-157, Enzo Life Sciences Inc.) by measuring the absorbance of the reaction products at 450 nm. The total glutathione (tGSH) and oxidized glutathione (GSSG) levels were measured using a glutathione (total) detection kit (cat. no. ADI-900-160) from Enzo Life Sciences Inc. by measuring the absorbance of the reaction products at 405 nm. The concentration of reduced glutathione (GSH) was calculated using the formula (GSH=tGSH-GSSG), which was provided in the kit protocol. The redox ratio was calculated using the formula GSH:GSSG=(tGSH-2GSSG)/GSSG, as described previously (29).

All data are reported as mean ± standard error of the mean. Statistical significance was analyzed using the Student's t test or, where applicable, two-way analysis of variance with Bonferroni post-hoc analysis for multiple group comparisons using GraphPad Prism software (version, 5.03; GraphPad Software Inc., La Jolla, CA, USA), and P<0.05 was considered statistically significant.

To evaluate the effect of NS seed extract on exercise durability, the exhaustive swimming test was performed using rats, which were pre-treated with either distilled water as a control or NS extracts for 21 days. As demonstrated in Fig. 1, the swimming time to exhaustion was significantly increased in the NS-treated group compared with control group (P<0.001; 24.6% increase vs. control). These data indicated that NS seed extract may prolong the swimming time in rats.

Exhaustive swimming resulted in significant decreases of pH (P<0.001), pO₂ (P<0.001) and O_2sat levels (P<0.001), but an increase of pCO₂ level (P<0.001), when compared with the pre-swimming control group. However, these changes were significantly attenuated by pre-treatment with NS seed extract compared with the post-swimming control group (P<0.01). Hb and Hct levels were slightly increased (P>0.05) following swimming in the control group. Notably, in pre-swimming and post-swimming of NS-pre-treated groups, these values had a tendency to increase compared with pre-swimming-control group, even though values in post-swimming group with pre-treatment of NS extract were not significantly changed compared with post-swimming control group (P>0.05; Table I). Finally, TP was markedly elevated in both control and NS-pre-treated groups following exhaustive swimming, when compared with pre-swimming control group. Moreover, there was no obvious difference in albumin levels between control and NS-treated groups following exhaustive swimming (Table I). These data indicated that NS seed extract could maintain the blood homeostasis following exhaustive swimming.

Fatigue can be evaluated by several important biochemical indicators, including glucose, lactate, LDH and CK. Exhaustive swimming caused depleted glucose, as an energy source, and the accumulation of lactate, LDH and CK (30). Thus, the authors examined the levels of fatigue-related blood biomarkers to test the anti-fatigue effect of NS seed extract. The exhaustive swimming led to a significant decrease in serum glucose level (from 127 to 103.2 mg/dl following exercise; P<0.001) but significant increases in lactate (3.5 to 5.5 mmol/l; P<0.001), LDH (202.4 to 811.6 IU/l; P<0.001) and CK (405.6 to 1288.4 IU/l; P<0.001) levels (Fig. 2) compared with the pre-swimming-control group. However, pre-treatment with NS extract significantly protected these exercise-induced alterations after exhaustive swimming (Fig. 2). The serum glucose level was significantly increased in the NS-treated group compared with control group following exhaustive swimming (P<0.01). Conversely, increased levels of serum lactate, LDH and CK, due to exhaustive swimming, were significantly attenuated by pre-treatment of NS extract (lactate, P<0.05; LDH and CK, P<0.001; Fig. 2). Taken together, the authors also demonstrated the anti-fatigue effects of NS extract on exhaustive swimming from the analysis of typical fatigue-related indicators (e.g., glucose, lactate, LDH and CK).

Glycogen content, which is main storage form of glucose, is an integral determining factor in fatigue following exhaustive swimming. Many studies have reported that glycogen is significantly depleted in both liver and muscles during exhaustive swimming (31). In the present study, following exhaustive swimming, glycogen levels in liver and g. muscle were significantly diminished compared with pre-swimming-control group (21.5 and 11.5% decreases in liver and g. muscle vs. control; P<0.001, respectively; Fig. 3). However, in NS extract-treated group, glycogen content was restored in both liver and g. muscle (39.4 and 10.2% increases in liver and g. muscle vs. swimming-control; P<0.001, respectively). In particular, the liver glycogen in NS-pre-treated-swimming group was significantly increased compared with control group (9.5% increase vs. control; P<0.05; Fig. 3A). These results demonstrated that NS extract administration may reserve glycogen in liver and g. muscle.

Oxidative stress occurs following exhaustive swimming, and subsequently may lead to pathology and clinical symptoms of fatigue (32). Therefore, the authors investigated the antioxidant activity of NS extract following exhaustive swimming by examining the SOD, MDA and serum redox ratio (GSH/GSSG) values as typical oxidative stress related parameters. Serum SOD level was significantly decreased in the swimming control-group, when compared with the control group (4.9% decrease vs. control; P<0.05). As expected, in the NS extract-pre-treated group, serum SOD level was significantly increased compared with the swimming control-group following exhaustive swimming (5.8% increase vs. swimming-control; P<0.01; Fig. 4A). Serum MDA level was dramatically increased following exhaustive swimming (28.1% increase vs. control; P<0.001). However, pre-treatment with NS extract inhibited the serum MDA level following exhaustive swimming (15.8% decrease vs. swimming-control; P<0.001; Fig. 4B). Similarly, the serum redox ratio (GSH:GSSG) was significantly decreased in the swimming-control group, when compared with the control group (10.8% decrease vs. control; P<0.05), but was increased in the exercise-NS extract-treated group (39.1% increase vs. swimming-control; P<0.001; Fig. 4C).

In addition, SOD levels in liver and g. muscle were significantly decreased compared with the control group following exhaustive swimming (21.9 and 6.0% decreases in liver and g. muscle vs. control; P<0.001, respectively; Fig. 5A and C). Notably, SOD levels in both tissues were significantly increased by pre-treatment of NS extract compared with the swimming-control-group (50.5 and 8.0% increases in liver and g. muscle vs. swimming-control; P<0.001, respectively; Fig. 5A and C). MDA levels in liver and g. muscle were significantly increased by pre-treatment of NS extract compared with the control group following exhaustive swimming (58.7 and 36.9% increases, in liver and g. muscle vs. control; P<0.001, respectively). However, when the NS extract was pre-treated, MDA levels in both tissues were significantly inhibited compared with exercise-control group (30.4 and 14.2% decreases in liver and g. muscle vs. swimming-control; P<0.001, respectively; Fig. 5B and D). These data suggested that NS extract may have a beneficial role against oxidative stress to alleviate physical fatigue following exercise.