Participants

Thirty-six healthy males (23 (sd 3) years; 1·79 (sd 0·06) m; 71·5 (sd 8·3) kg) volunteered to participate in this parallel-group, double-blind, randomised controlled trial (participants’ characteristics are presented in Table 1). Participants were recreationally active and generally performed between 2 and 4 exercise sessions per week in various sports (e.g. soccer, basketball, weight lifting, running, cycling, etc.) but were not involved in any structured progressive exercise training regimen. The present study was part of a larger trial registered at the Netherlands Trial Register (NTR6548, https://www.trialregister.nl/trial/6364) and was conducted between June 2017 and April 2019 at Maastricht University in Maastricht, the Netherlands (see supplementary material, Supplemental Figure 1 for the CONSORT (Consolidated Standards of Reporting Trials) flow diagram). All participants were informed about the purpose of the study, the experimental procedures and possible risks before providing informed written consent to participate. The procedures followed were in accordance with the ethical standards of the medical ethics committee of Maastricht University Medical Centre + (METC 173001), and in accordance with the Helsinki Declaration of 1975 as revised in October 2013. The study was independently monitored and audited by the Clinical Trial Centre Maastricht.

Table 1. Participants’ characteristics

Values represent mean and standard deviation. n = 12 per nutritional intervention group. MILK: 30 g of milk protein, WHEAT+MILK: 15 g of wheat protein plus 15 g of milk protein, WHEAT: 30 g of wheat protein. Independent-samples t test for MILK v. WHEAT and MILK v. WHEAT+MILK all P > 0·05.

Preliminary testing

Participants aged 18–35 years with BMI > 18·5 and < 27·5 kg·m⁻² underwent an initial screening session to assess eligibility. Height, weight, blood pressure and body composition (by dual-energy X-ray absorptiometry; Discovery A, Hologic; (National Health and Nutrition Examination Survey – Body Composition Analysis (NHANES BCA) enabled) were determined. Participants were deemed healthy based on their responses to a medical questionnaire. The screening sessions and experimental trials were separated by at least 3 d.

Study design

Participants were randomly assigned to ingest a 400 ml beverage containing either 30 g milk protein concentrate (MILK), 30 g wheat protein hydrolysate (WHEAT), or 15 g wheat protein hydrolysate plus 15 g milk protein concentrate (WHEAT+MILK). After beverage ingestion, the bottle was rinsed with 150 ml of water, which was also ingested by the participants. Milk protein concentrate (Refit MPC80) was obtained from FrieslandCampina and wheat protein hydrolysate (Meripro 500) was supplied by Tereos Syral. Participants were allocated to a treatment according to a block randomisation list (blocks of 7) performed using a computerised randomiser (http://www.randomization.com/). An independent researcher was responsible for random assignment (n = 12 per group) and preparation of the study treatment beverages, which were sequentially numbered according to subject number. The beverages were prepared in non-transparent protein-shakers.

Diet and physical activity

Participants refrained from sports and strenuous physical activities (e.g. lifting heavy weights), and alcohol consumption for 3 d prior to the experimental trial. In addition, all participants were instructed to complete a food and activity record for 3 d prior to the experimental trial (see online supplementary material, Supplemental Table S1 for an overview of participants’ habitual food intake in the 3 d prior to the experimental trial). The evening before the trial, all participants consumed a standardised meal containing 2·8 MJ of energy, with 65 % energy provided as carbohydrate, 20 % as fat and 15 % as protein, before 22.00 after which they remained fasted.

Experimental protocol

At about 07.30, participants arrived at the laboratory in an overnight post-absorptive state. A cannula was inserted into an antecubital vein for stable isotope AA infusion. A second cannula was inserted retrogradely into a dorsal hand vein on the contralateral arm for arterialised blood sampling. To obtain arterialised blood samples, the hand was placed in a hot box (60 °C) for 10 min prior to blood sample collection.

After taking a baseline blood sample (t = –180 min), the plasma phenylalanine pool was primed with a single dose of L-[ring-¹³C₆]-phenylalanine (2·25 µmol·kg⁻¹). Thereafter, a continuous intravenous infusion of L-[ring-¹³C₆]-phenylalanine (0·05 µmol·kg⁻¹·min⁻¹) was initiated (t = –180 min) using a calibrated IVAC 598 pump. Subsequently, arterialised blood samples were collected at t = –90, –60 and –30 min. At t = 0 min, an arterialised blood sample was obtained as well as a muscle biopsy from the M. vastus lateralis. Immediately following the muscle biopsy, participants ingested a 400 ml beverage corresponding to their randomised treatment allocation, that is, MILK (n = 12), WHEAT (n = 12), or WHEAT+MILK (n = 12). To minimise dilution of the steady-state plasma L-[ring-¹³C₆]-phenylalanine precursor pool, the phenylalanine content of each protein drink was enriched with 3·85 % free, crystalline L-[ring-¹³C₆]-phenylalanine^{(Reference Churchward-Venne, Pinckaers and Smeets21,Reference Churchward-Venne, Pinckaers and Smeets27)} . Arterialised blood samples were then collected at t = 15, 30, 45, 60, 90, 120, 150, 180, 210, 240 and 300 min after protein ingestion in the post-prandial period. Blood samples were collected into EDTA-containing tubes and centrifuged at 1200 g for 10 min at 4 °C. Aliquots of plasma were frozen in liquid nitrogen and stored at –80 °C. The second and third muscle biopsy from the M. vastus lateralis were collected at t = 120 and t = 300 min to determine post-prandial skeletal muscle protein synthesis rates over the 0–120, 120–300 and 0–300 min post-prandial period. Muscle biopsy collection was alternated between legs and obtained with the use of a 5-mm Bergström needle^{(Reference Bergstrom28)}, custom-adapted for manual suction. Samples were obtained from separate incisions from the middle region of the M. vastus lateralis, about 15 cm above the patella and about 3 cm below entry through the fascia. Local anesthetic (1 % Xylocaine with adrenaline 1:100 000) was applied to numb the skin and fascia. Muscle samples were freed from any visible non-muscle material, immediately frozen in liquid nitrogen, and stored at –80 °C until further processing. When the experimental protocol was complete, cannulae were removed and participants were provided with food and monitored for about 30 min before leaving the laboratory. For a schematic representation of the infusion protocol, see Fig. 1.

Fig. 1. Schematic representation of the experimental design.

Protein powder analysis

Batch-specific N contents of both milk protein concentrate and wheat protein hydrolysate were provided by the manufacturer. The protein content of the milk protein was determined as N content × 6·38, and the protein content of wheat protein powder was determined as N content × 5·7^{(Reference Jones29,Reference Mariotti, Tome and Mirand30)} . AA contents of the protein powders were determined by acid hydrolysis in triplicate. Specifically, the AA were liberated from the protein powders (about 4 mg) by adding 2 ml of 6M HCl and heating to 110 °C for 12 h. The hydrolysed free AA were subsequently dried under a N stream while heated to 120 °C. Before analysis using ultra-performance liquid chromatography (UPLC)-MS (ACQUITY UPLC H-Class with QDa; Waters), the hydrolysate was dissolved in 5 ml of 0·1 M HCl and 20 µl of AccQ/Tag derivatising reagent solution (Waters) was added as described below for the plasma AA concentration analysis. The AA composition of the protein powders and the protein blend are presented in Table 2.

Table 2. Protein drink amino acid composition

Values for amino acid contents are in grams per 30 g of protein. MILK: 30 g of milk protein, WHEAT+MILK: 15 g of wheat protein plus 15 g of milk protein, WHEAT: 30 g of wheat protein.

TAA, total amino acid; EAA, essential amino acid; BCAA, branched chain amino acid

* Values are obtained by averaging the measured values for wheat and milk protein.

† Protein as N content × 6·38.

‡ Protein as N content × 5·7.

Plasma analysis

Plasma glucose and insulin concentrations were analysed using commercially available kits (GLUC3, Roche, Ref: 05168791190, and immunologic, Roche, Ref: 12017547122, respectively). Plasma AA concentrations were determined by UPLC-MS. Specifically, 50 µl of blood plasma was deproteinised using 100 µl of 10 % SSA with 50 µM of MSK-A2 internal standard (Cambridge Isotope Laboratories). Subsequently, 50 µl of ultra-pure demineralised water was added and samples were centrifuged. After centrifugation, 10 µl of supernatant was added to 70 µl of Borate reaction buffer (Waters). In addition, 20 µl of AccQ/Tag derivatising reagent solution (Waters) was added after which the solution was heated to 55 °C for 10 min. Of this 100-µl derivative, 1 µl was injected and measured using UPLC-MS.

Plasma L-[ring-¹³C₆]-phenylalanine enrichments were determined by GC-MS (Agilent 7890A GC/5975C MSD; Agilent Technologies). Specifically, the plasma was deproteinised on ice with dry 5-sulfosalicyclic acid. Free AA were purified using cation exchange resin columns (AG 50W-X8, mesh size: 100–200, ionic form: hydrogen (Bio-Rad Laboratories)). The free AA were converted to their tert-butyl dimethylsilyl derivative before analysis by GC-MS using selected ion monitoring of masses 336 and 342 for unlabelled and [ring-¹³C₆]-labelled phenylalanine, respectively. Standard regression curves were applied from a series of known standard enrichment values against the measured values to assess the linearity of the mass spectrometer and to account for any isotope fractionation which may have occurred during the analysis.

Basal muscle protein synthesis rates were assessed to confirm that protein ingestion increases muscle protein synthesis rates. The single biopsy approach was applied to assess post-absorptive muscle protein synthesis rates without the need to collect an additional muscle biopsy^{(Reference Burd, Pennings and Groen31)}. In short, plasma protein obtained prior to tracer infusion (t = –180 min) was used to determine background L-[ring-¹³C₆]-phenylalanine enrichments. For this purpose, the plasma sample was precipitated by adding perchloric acid. Subsequently, similarly as for the myofibrillar protein fraction, the denaturised plasma protein pellet was hydrolysed, passed over a cation exchange resin column (AG 50W-X8, mesh size: 100–200, ionic form: hydrogen (Bio-Rad Laboratories)), and the resulting AA samples were derivatised to their N(O,S)-ethoxycarbonyl-ethylesters before being measured by GC-combustion-isotope ratio mass spectrometry (GC-C-IRMS; Mat 253, Thermo Scientific) using a DB5MS (30 m) column (Agilent technologies), as explained below.

Muscle analysis

A piece of wet muscle (about 50–70 mg) was homogenised on ice using a Teflon pestle in ice-cold homogenisation buffer (7 µl/mg; 67 mM sucrose, 50 mM TRIS/HCl, 50 mM KCl, 10 mM EDTA) containing Complete Mini protease inhibitor cocktail and PhosSTOP (Roche Applied Science). After about 3 min of hand homogenisation, the homogenate was centrifuged at 2200 g for 5 min at 4 °C to precipitate the myofibrillar proteins. The protein pellet was washed once with MilliQ water and centrifuged at 250 g for 10 min at 4 °C. The myofibrillar proteins were solubilised by adding 1 ml of 0·3 M NaOH and heating to 50 °C for 30 min with vortex mixing every 10 min. Samples were centrifuged at 11 000 g for 5 min at 4 °C and the supernatant containing the myofibrillar protein-enriched fraction was collected. The collagen pellets were washed once with 0·3 M NaOH and centrifuged at 11 000 g for 5 min at 4 °C. The resulting supernatant was added to the already collected myofibrillar protein-enriched fraction and the collagen pellets were discarded. Myofibrillar proteins were precipitated by the addition of 1 ml of 1 M perchloric acid and centrifuged at 800 g for 10 min at 4 °C. The myofibrillar protein-enriched fraction was washed twice with 70 % ethanol and centrifuged at 450 g . The AA were liberated from the myofibrillar protein-enriched fraction by adding 2 ml of 6 M HCl and heating to 110 °C for 16 h. The hydrolysed myofibrillar protein fractions were dried under a N stream while heated to 120 °C. The dried myofibrillar protein fraction was dissolved in a 50 % acetic acid solution. The AA from the myofibrillar protein fraction were passed over a cation exchange resin column (AG 50W-X8, mesh size: 100–200, ionic form: hydrogen (Bio-Rad Laboratories). Subsequently, the purified AA solution was dried under a N stream at room temperature, followed by derivatization to their N(O,S)-ethoxycarbonyl-ethylesters. The ratio of ¹³C/¹²C of myofibrillar protein-bound phenylalanine was determined using GC-C-IRMS by monitoring ion masses 44, 45 and 46. Standard regression curves were applied from a series of known standard enrichment values against the measured values to assess the linearity of the mass spectrometer and to account for any isotope fractionation which may have occurred during the analysis.

Muscle intra-cellular enrichments were determined from a separate piece of muscle. Specifically, a piece of wet muscle (about 50–70 mg) was freeze-dried for 48 h. Collagen, excessive blood and other non-muscle materials were subsequently removed from the muscle fibres under a light microscope. The isolated muscle fibre mass was weighed and 35 volumes (7× wet weight of isolated muscle fibres × wet-to-dry ratio 5:1) of ice-cold 2 % perchloric acid was added. Thereafter, the tissue was homogenised by sonification and centrifuged to separate the supernatant from the protein. The supernatants containing the muscle intra-cellular free AA were purified, and derivatised before analysis by GC-MS, similarly as for the plasma L-[ring ¹³C₆]-phenylalanine enrichments.

Calculations

Fractional myofibrillar protein synthesis rates (%·h⁻¹) were calculated by the standard precursor-product equation^{(Reference Schierbeek32)}:

$$FSR = \left( {{{({E_{b2}} - {E_{b1}})} \over {({E_{precursor}} \cdot t)}}} \right) \cdot 100$$

where E _b is the increment in myofibrillar protein-bound L-[ring-¹³C₆]-phenylalanine enrichment (mole % excess, MPE) during the tracer incorporation period, and t is the tracer incorporation time in hours. Weighted mean plasma L-[ring-¹³C₆]-phenylalanine enrichments were calculated by taking the measured enrichment between consecutive time points and correcting for the time between these sampling time points (E _precursor). For calculation of post-prandial fractional synthetic rate (FSR), skeletal muscle biopsy samples at t = 0, 120 and 300 min were used. For the calculation of basal FSR, E_b2 represented the protein-bound L-[ring-¹³C₆]-phenylalanine enrichments in muscle at t = 0 min, and E_b1 represented the protein-bound L-[ring-¹³C₆]-phenylalanine enrichments in plasma protein at t = −180 min.

Net incremental AUC (iAUC) was determined for plasma AA concentrations during the 5-h post-prandial period following protein ingestion. The iAUC was calculated using the trapezoid rule, with plasma concentrations before beverage ingestion (t = 0 min) serving as baseline.

Outcome measures

Myofibrillar FSR over the entire (i.e. 0–300 min) post-prandial period, comparing MILK v. WHEAT and MILK v. WHEAT+MILK was defined as the primary outcome measure. Secondary outcome measures were myofibrillar FSR in the early (i.e. 0–120 min) and late (i.e. 120–300 min) post-prandial period, plasma glucose, insulin, and AA concentrations and plasma AA iAUC, comparing MILK v. WHEAT and MILK v. WHEAT+MILK. Plasma glucose, insulin, and AA peak concentrations and time to peak were tertiary outcomes, comparing MILK v. WHEAT and MILK v. WHEAT+MILK.

Statistical analysis

A power calculation was performed with differences in post-prandial myofibrillar FSR between two treatments as primary outcome measure. A sample size of twelve participants per treatment, including a 10 % dropout rate, was calculated using a power of 80 %, a significance level of 0·05, a standard deviation of 0·0065 %·h⁻¹ and a difference in FSR of 0·008 %·h⁻¹ between treatments (or about 20 % when expressed as a relative difference). Participant characteristics were analysed by independent-samples t test for MILK v. WHEAT and MILK v. WHEAT+MILK. Plasma glucose, insulin, and AA concentrations and AA enrichments were analysed by a two-way (time × treatment) repeated-measures ANOVA for MILK v. WHEAT and MILK v. WHEAT+MILK. Bonferroni post hoc analysis was performed if a significant F ratio was found to isolate specific differences. Plasma glucose, insulin and AA concentrations, expressed as peak values, time to peak and iAUC, were analysed by independent-samples t test for MILK v. WHEAT and MILK v. WHEAT+MILK. Basal post-absorptive and post-prandial myofibrillar protein synthesis rates during the early (0–120 min) and entire (0–300 min) post-prandial period were analysed by independent-samples t test for MILK v. WHEAT and MILK v. WHEAT+MILK. Statistical analyses were performed with a software package (IBM SPSS statistics for Windows, version 26.0, IBM Corp.). Means were considered to be significantly different for P values < 0·05. Data are expressed as means values and standard deviations.