Eicosapentaenoic and docosahexaenoic acids-rich fish oil supplementation attenuates strength loss and limited joint range of motion after eccentric contractions: a randomized, double-blind, placebo-controlled, parallel-group trial

A total of 24 Japanese healthy men (age, 19.5 ± 0.8 years; height, 174.4 ± 6.0 cm; weight, 65.3 ± 7.7 kg; body fat, 13.3 ± 3.1 %) were recruited for this study. They were allergic to fish and resistance training and requested to avoid participation in other clinical trials and interventions such as massage, stretching, strenuous exercise, excessive consumption of food or alcohol, and any supplement or medication during the experimental period. All participants were provided with detailed explanations of the study protocol prior to participation and signed an informed consent form in accordance with the Declaration of Helsinki before being enrolled in this study. This study was approved by the Ethics Committee for Human Experiments at Juntendo University (ID: 26–113) and has been registered at the University Hospital Medical Information Network Clinical Trials Registry (UMIN-CTR, identifier: UMIN000016149). The estimation was based on the effect size of 1, alpha level of 0.05, and a power (1−b) of 0.80 for the comparison EPA group and PL group following ECC, which showed that at least ten participants were necessary (G*power, version 3.0.10).

The study was performed by a double-blind, placebo-controlled, parallel-group trial design. All subjects were randomly assigned to two groups in such a manner as to minimize the inter-group differences in age, body fat, BMI, and maximal voluntary isometric contraction (MVC) torque, and they consumed either EPA and DHA (EPA, n = 12; age, 19.4 ± 0.7 years; height, 174.4 ± 5.6 cm; weight, 64.3 ± 7.7 kg; body fat, 13.0 ± 3.5 %; MVC, 58.6 ± 14.9 Nm) or placebo (PL, n = 12; age, 19.5 ± 0.8 years; height, 174.3 ± 6.7 cm; weight, 66.2 ± 8.0 kg; body fat, 13.6 ± 2.8 %; MVC, 58.0 ± 11.6 Nm) for 8 weeks prior to the exercise experiment and continued it until 5 days after the exercise. Sequence allocation concealment and blinding to subjects and researchers were maintained during treatment. Since it has been reported that the compensation of EPA and DHA concentration into the myocardium is needed for the ingestion of fish oil for 30–60 days (Metcalf et al. 2007), the duration of the total ingestion period was 62 days (including the exercise day). On the day of exercise testing, MVC torque, range of motion of the elbow joint (ROM), upper arm circumference, muscle soreness assessed by a visual analog scale (VAS), and fasting blood samples were measured in the non-dominant arm before exercise. Immediately after baseline measurements, ECC in the non-dominant arm as with the other measurement was performed in each subject. All measurements were performed immediately before, immediately after, and 1, 2, 3, and 5 days after exercise. Measurements were performed in a room maintained at 24−26 °C. In addition, we surveyed the nutrition status of all subjects prior to supplement consumption (8 weeks before the exercise experiment) and after experimental testing of the food frequency questionnaire based on food groups (FFQg, version 3.5, Kenpakusha, Tokyo, Japan). The outcome measures were MVC torque, ROM, upper arm circumference, muscle soreness, and blood serum markers. In addition, we also measured serum fatty acids including EPA, DHA, arachidonic acid (AA), and dihomo-gamma-linolenic acid (DGLA). Based on the two baseline measures of MVC torque, ROM, upper arm circumference, and muscle soreness (before exercise and different day), the test–retest reliability of the measures was examined.

The EPA group consumed eight 300 mg EPA and 130 mg DHA-rich fish oil softgel capsules (Nippon Suisan Kaisha Ltd., Tokyo, Japan) per day (containing 600 mg EPA and 260 mg DHA in a total of 2400 mg). The PL group consumed eight 300 mg corn oil softgel capsules (Nippon Suisan Kaisha Ltd., Tokyo, Japan) per day (not containing EPA and DHA in a total of 2400 mg). Subjects consumed the supplements 30 min after meals with water.

Each subject was seated in the chair of an isokinetic dynamometer (Biodex Multi-Joint System 3, NY, USA) with one arm set at a shoulder joint angle of 45° flexion, and the elbow joint aligned with the rotation axis of the isokinetic dynamometer. The lever arm of the isokinetic dynamometer was secured to the wrist of subjects in a supinated position. ECC consisted of five sets of six maximal voluntary eccentric contractions of the elbow flexors at a constant velocity of 30°/s for the range of motion from 90° flexion to 0° (full extension). Subjects were verbally encouraged to maximally resist throughout the ROM for 3 s. The isokinetic dynamometer returned the arm to the 90° flexed position at a constant velocity of 30°/s, providing 3 s passive recovery between contractions. The measurements of torque produced during eccentric contractions were stored in a computer connected to the isokinetic dynamometer, and work output and peak torque were calculated later. These measurements were based on a previous study (Chen et al. 2011).

MVC torque was measured on the same apparatus and positioning as described for eccentric exercise. Subjects performed two 5-s MVCs at 90° elbow joint angle with a 15-s rest between contractions. The peak torque of the two contractions was used as the MVC torque as described in our previous study (Tsuchiya et al. 2015). The test–retest reliability of the MVC measures based on coefficient of variation (CV) was 3.9 %.

To examine the elbow joint ROM, two elbow joint angles (extended and flexed joint angles) were measured using a goniometer (Takase Medical, Tokyo, Japan). The extended joint angle was recorded when subjects attempted to fully extend the joint, with the elbow held by their side and the hand in supination. The flexed joint angle was determined when subjects attempted to fully flex the joint from an equally fully extended position with the hand supinated. ROM was calculated by subtracting the flexed joint angle from the extended joint angle (Tsuchiya et al. 2015). The test–retest reliability of the ROM measures based on CV was 4.2 %.

Upper arm circumference was assessed at 3, 5, 7, 9, and 11 cm above the elbow joint using a tape measure while subjects were standing with the arms relaxed by their side. The mean value of five measurements was used for analysis (Nosaka et al. 2005). Measurement marks were maintained during the experimental period using a semi-permanent ink marker, and a well-trained investigator took the measurements. The average value of three measurements was used for further analysis. The test–retest reliability of the circumference measurements for the five sites based on CV was 2.2–3.4 %.

Muscle soreness was assessed using a 100-mm VAS in which 0 indicates ‘‘no pain’’ and 100 is the ‘‘worst pain imaginable’’. Each subject was asked to indicate the pain level on the scale when an investigator palpated the biceps brachii, brachialis, or brachioradialis, respectively, using a thumb while subjects relaxed with their arms in the natural position. All tests were conducted by the same investigator who had been trained to apply the same pressure over time and between subjects. The test–retest reliability of the VAS measures for the three muscles based on CV was 0–4.7 %.

Subjects fasted for 8 h prior to blood samples being taken from the forearm by a trained doctor. Blood samples were allowed to clot at room temperature (25 °C) and then centrifuged at 3000 rpm for 10 min at 4 °C. Serum was extracted and stored at −20 °C until analysis. The serum levels of CK, Mb, IL-6, TNF-α, and four fatty acids (DGLA, AA, EPA, DHA) were measured. Serum CK levels were measured according to the Japan Society of Clinical Chemistry Standardized Method. Serum Mb and IL-6 levels were measured by chemiluminescence enzyme immunoassay (CLEIA), and serum TNF-α levels were measured using an enzyme-linked immunosorbent assay (ELISA). Serum fatty acid levels were measured using gas chromatography spectrometry (GC). The test–retest reliability of the CK, Mb, IL-6, and TNF-α measurements based on CV was 3.8, 2.8, 2.9, and 11.4 %, respectively. Also, that of the DGLA, AA, EPA, and DHA measurements based on CV were 5.6, 4.9, 5.1, and 6.6 %, respectively.

No significant difference in work output (Fig. 1a) or peak torque (Fig. 1b) during any set of ECC was observed between the two groups.

MVC torque value was indicated by relative change compared with pre ECC value as 100 % (EPA group, 58.6 ± 14.9 Nm; PL group, 58.0 ± 11.6 Nm). MVC torque (Fig. 2a) in the PL group significantly decreased from immediately after to 5 days after exercise compared with pre-exercise levels (post, day 1, day 2, day 3, and day 5, p < 0.05). MCV torque in the EPA group decreased immediately after exercise compared with pre-exercise levels (p < 0.05). MVC was significantly higher in the EPA group than in the PL group at 2, 3, and 5 days after exercise [day 2; PL 78.4 ± 10.4 %, EPA 95.5 ± 20.1 %, Cohen’s d (d) = 1.04, 95 % confidence interval (CI) 0.15–1.85, day 3; PL 82.6 ± 6.8 %, EPA 98.7 ± 15.0 %, d = 1.39, CI 0.45–2.22, and day 5; PL 85.1 ± 11.4 %, EPA 101.3 ± 14.0 %, d = 1.27, CI 0.35–2.10, p < 0.05].

Figure 2b showed the values of ROM by relative change compared with pre ECC value as 100 % (EPA group, 127.3° ± 7.5°; PL group, 130.6° ± 10.4°). Although no significant decrease in elbow ROM from pre-exercise values was observed in the EPA group, a significant decrease in the PL group was observed immediately after exercise (reduction of 18.0 ± 6.1 %, p < 0.05) and remained lower than baseline levels at 1, 2, and 3 days (p < 0.05). Elbow ROM in the EPA group was significantly greater than that in the PL group from immediately after exercise to 3 days after exercise (post; PL 84.0 ± 7.2 %, EPA 96.4 ± 10.9 %, d = 1.88, CI 0.87–2.77, day 1; PL 89.0 ± 6.3 %, EPA 99.0 ± 8.1 %, d = 1.50, CI 0.55–2.35, day 2; PL 88.0 ± 7.1 %, EPA 97.6 ± 8.8 %, d = 1.11, CI 0.22–1.93, and day 3; PL 88.5 ± 10.9 %, EPA 99.6 ± 6.0 %, d = 1.01, CI 0.13–1.83, p < 0.05). ROM was also evaluated as absolute values in degrees. At post-ECC, days 2 and 3, elbow ROM degree was significantly different between the two groups. The degree of ROM indicated 111.5° ± 14.6° vs 120.3° ± 13.2° at post-ECC, 116.4° ± 10.1° vs 121.6° ± 9.5° at day 2, and 116.7° ± 11.7° vs 125.0° ± 7.2° at day 3 (PL group vs EPA group, respectively).

Upper arm circumference value was indicated by the change rate compared with the pre-ECC value as 100 % (EPA group, 25.0 ± 1.5 cm; PL group, 26.0 ± 1.7 cm). No significant difference in the upper arm circumference from pre-exercise values was observed in either group (EPA, 101.8 ± 1.1 %; PL, 101.3 ± 1.9 %). No significant difference between the two groups was observed at any time point (Fig. 2c).

Greater muscle soreness developed at the biceps brachii and brachialis at 1, 2, and 3 days after exercise compared with pre-exercise values in the PL group (Fig. 3a, b). In the EPA group, greater muscle soreness developed at the biceps brachii at 1, 2, and 3 days after exercise and at the brachialis at 2 days after exercise compared with pre-exercise values (Fig. 3a, b). Significantly greater muscle soreness at the brachialis was observed in the PL group compared with the EPA group at 3 days after exercise (PL, 34.2 ± 15.3 mm vs EPA, 12.7 ± 16.5 mm, d = 1.46, CI 0.52–2.31, p < 0.05). On the other hand, no significant increase in muscle soreness at the brachioradialis from pre-exercise values was observed in either group, with no significant difference between groups observed at any time point (Fig. 3c).

No significant differences in AA and DHA from pre-exercise values were observed in either group, with no significant differences between groups at any time point (data not shown). No significant difference in DGLA from pre-exercise values was observed in either group; however, significantly higher levels were observed in the PL group than the EPA group at 2 and 3 days after exercise (p < 0.05). On the other hand, EPA was significantly higher in the EPA group than in the PL group from before exercise to 3 days after exercise (pre; d = 0.52, CI 0.31–1.31, post; d = 0.50, CI 0.33–1.29, day 1; d = 0.80, CI 0.06–1.60, day 2; d = 0.65, CI 0.19–1.44, and day 3; d = 0.64, CI 0.20–1.44, p < 0.05).

Although serum IL-6 levels in the PL group were significantly increased at 3 days after exercise compared with pre-exercise vales (Fig. 4a, p < 0.05), no significant difference in serum IL-6 levels after exercise compared with pre-exercise values was observed in the EPA group. Serum IL-6 levels were significantly higher in the PL group than the EPA group at 3 days after exercise (PL, 1.8 ± 1.1 μg/ml vs EPA, 0.8 ± 0.4 μg/ml, d = 1.17, CI 0.27–1.99, p < 0.05). In contrast, no significant difference in serum TNF-α levels after exercise compared with pre-exercise values was observed in either group, with no significant difference observed between groups (Fig. 4b).

Serum Mb levels in the PL group were significantly increased at 3 days after exercise compared with pre-exercise values (Fig. 2d, p < 0.05); however, no significant difference after exercise compared with pre-exercise values was observed in the EPA group. No significant differences in serum CK levels after exercise compared with pre-exercise values were observed in either group, with no significant difference observed between groups (Fig. 2e).