Production of n-3 very-long-chain-PUFA concentrates for Atlantic salmon feeding trial and cell culture experiments

Two n-3 VLC-PUFA concentrates, VLC-Conc1 and VLC-Conc2, were made from an anchovy fish oil distillation fraction by hydrolysis, precipitation with LiOH and distillation^{(Reference Svensen and Breivik30)} as previously described^{(Reference Torrissen, Svensen and Stoknes29)}. Both VLC-Conc1 and VLC-Conc2 were produced by Epax Norway AS. VLC-Conc1 was used for the salmon feeding trial, and VLC-Conc2 was used for the cell culture experiments. A synthetic VLC-PUFA 26:6 n-3, custom-made and purchased from BOC Sciences, was used in the cell culture experiments using primary keratocytes from Atlantic salmon. The fatty acid composition of the concentrates is presented in Table 1. The purpose of using different concentrates in the cell culture experiments and the salmon feeding trial was to single out the VLC-PUFA effect from effects of other fatty acids in the in vitro studies. Therefore, either a VLC-PUFA concentrate enriched with only unsaturated fatty acids with > 22 carbon atoms was used or a pure 26:6 n-3 substrate. The salmon feed, on the other hand, already consisted of many fatty acids other than the VLC-PUFA, and therefore there is no need to use a VLC-PUFA concentrate devoid of SFA and ≤ 22 carbon MUFA and PUFA.

Table 1. Fatty acid composition of VLC-PUFA concentrates (VLC-Conc1 and VLC-Conc2), presented as percentage (%) of total fatty acids*

ND, not detected; VLC-PUFA, very-long-chain PUFA.

* Analytical methods used detects fatty acids ≤ C30.

† Others include 16:4, 24:2, 26:3 and 28:2.

Dietary supplementation of Atlantic salmon with increasing levels of n-3 very-long-chain-PUFA

A 4-week in vivo feeding trial using Atlantic salmon (Salmo Breed) was conducted in freshwater tanks at Nofima’s Aquaculture Research facilities at Sunndalsøra, Norway. Five different experimental diets that were produced at the Nofima Feed Technology centre in Bergen, Norway, were tested using three tanks per diet group and 100 fish per tank. During the study period, the fish grew from an initial weight of approximately 6 g to a final weight of approximately 11 g. The basal diet consisted of 50 % fishmeal and 10 % each of wheat, wheat gluten, and soya protein concentrate, in addition to minerals and vitamin mixture (Table 2). The diets were isoenergetic and contained 50 % protein and 20 % lipid. The five different experimental diets were supplemented with increasing levels (0–10 %) of VLC-Conc1, while levels of EPA and DHA were kept constant. The amount of fish oil was reduced from 13 % to 0 % as the amount of VLC-Conc1 and rapeseed oil increased in the diets. The composition of the basal diet was identical for all groups, except for the fatty acid composition of the oil coating of the basal diet, which was coated on the pellets with a vacuum coater in the final production step. The ingredient and fatty acid compositions of the diets are shown in Tables 2 and 3, respectively. We aimed at optimal voluntary feed intake in each tank. By controlled over-feeding, we secured that all fish had access to sufficient amount of feed throughout the experiment.

Table 2. Ingredient composition of the diets, presented as g/100 g feed. Diet groups are named according to the percentage VLC-Conc1 included in the feed

VLC-PUFA, very-long-chain PUFA.

* Vedde AS (Norway).

† Norgesmøllene AS (Norway).

‡ Tereos Syral (France).

§ Agrokorn (Germany).

|| Vilomix (Norway).

¶ Normin (Norway). Provided per 100 grams of feed: vitamin D, 300 mg; vitamin E, 16 mg; thiamin, 2 mg; riboflavin, 3 mg; pyridoxine-HCl, 3 mg; vitamin C, 20 mg; calcium d-pantothenate, 6 mg; biotin, 0·11 mg; folic acid, 1 mg; niacin, 20·1 mg; cobalamin, 0·005 mg; vitamin K3, 2 mg.

** Normin (Norway).

†† DSM (The Netherlands).

‡‡ Normin (Norway), Provided per 100 g of feed: K, 80 mg; Mg, 75 mg; Zn, 12 mg; Fe, 6 mg; Mn, 3 mg; Cu, 0·6 mg; Se, 0·03 mg.

§§ Emmelev (Denmark).

|||| Epax Norway AS (Norway).

¶¶ Epax Norway AS (Norway). 0·00, 2·50, 5·00, 7·50 and 10·00 of concentrate corresponds to 0·00, 0·54, 1·09, 1·63 and 2·18 VLC-PUFA in g/100 g feed, respectively.

Table 3. Fatty acid composition of the diets, presented as grams of fatty acid/100 g feed. Diet groups are named according to the percentage VLC-Conc1 included in the feed

VLC-PUFA, very-long-chain PUFA.

* Values calculated based on inclusion levels of VLC-Conc1 in the feed.

Growth rates were calculated based on the average weights of the fish in each tank as follows, where W₀ represents the starting weight (g), W₁ represents the final weight (g), t represents the number of days, and d° represents the degree-days (sum of average temperature for all feeding days):

$${\rm{Specific}}\,{\rm{growth}}\,{\rm{rate}}({\rm{SGR}}) = \left[ {{{\rm{e}}^{(\ln {{\rm{W}}_1}{\rm{\;}} - \ln {{\rm{W}}_0}/{\rm{t}})}} - 1} \right] \times 100$$

$${\rm{Thermal}}\,{\rm{growth}}\,{\rm{coefficient}}\,\left( {{\rm{TGC}}} \right) = \left( {{W_1}^{{1 \over 3}}-{W_0}^{{1 \over 3}}} \right) \times {{1000} \over d}^\circ $$

Sampling and sample preparation

Ten fish were randomly selected from each tank and euthanised by overdose (0·05–0·08 g/l) of anaesthetic (Metacain, MS-222) at three different time points: start of the trial (0 d); midway (18 d); and end of the trial (28 d). Standardised tissue samples of skin from the area above the lateral line and underneath the dorsal fin were taken from ten fish and fixed in neutral buffered 10 % formalin solution (Sigma-Aldrich). Skin samples were also excised and frozen in liquid N₂ before storing at –80°C until used later to analyse lipid composition. At the final sampling, all the fish in each tank were bulk-weighed.

Histology

Skin samples taken at the start, midway and final sampling (days 0, 18 and 28, respectively) were dissected and placed in tissue-embedding cassettes (Simport). Tissue processing was performed using an automated tissue processor (TP1020, Leica Biosystems, Nussloch GmbH) in which the samples were dehydrated using 100 % alcohol and a clearent xylene bath, before infiltration in melted paraffin at 60°C (Merck KGaA). Paraffin-embedded tissue samples were cut into 5-µm sections using a Microtome (Leica RM 2165), mounted on polysin-coated slides (VWR, Avantor) and dried overnight at 37°C. The sections were deparaffinised and rehydrated, and staining was performed using an automated special stainer (Autostainer XL Leica Biosystems, Nussloch GmbH Paraffin sections were stained with haematoxylin–eosin (H&E) and Von Kossa (Sigma Aldrich). All slides were examined using a light microscope slide scanner (Leica Microsystems) and manually evaluated using an Aperio Image Scope (Leica).

In vitro cell culture of primary Atlantic keratocytes and human dermal fibroblasts

Fatty acid composition analysis

For the fatty acid composition analysis, total lipids were extracted from homogenised tissue or sonicated extracts of cells following the method previously described by Folch et al. ^{(Reference Folch, Lees and Sloane Stanley33)}. For skin tissue, three pooled samples of ten individual tissue samples (ten fish from each of the triplicate tanks per diet group, thirty fish in total) were analysed for lipid composition per diet group. For cells, three individual cell culture flasks per treatment group were analysed.

To determine the lipid class composition of the skin tissue, the Folch chloroform lipid extract was evaporated under N₂ gas, and the residual lipid extract was redissolved in hexane (VWR). Phospholipids (PL) were separated by TLC using the method described by Bou et al^{(Reference Bou, Berge and Baeverfjord34)}. In brief, TLC plates (Watman K6 – Silica Gel 60 Å, 0·25-mm film thickness, 20 × 20 cm; VWR) were preconditioned in methanol in a separation chamber under a fume hood and dried at 120°C for 20 min. Lipid fractions were then applied to the plates for migration and placed in a TLC separation chamber. PL were separated using a mixture of petroleum ether, diethyl ether and acetic acid (113:20:2, v/v/v) as the mobile phase. The plates were then dried in a fume hood, sprayed with 2 % 2–7-dichlorofluorescein in ethanol and dried again. UV light (366 nm) was used to detect the lipid classes, which appeared as yellow spots when placed under UV light. Spots were marked while under the UV light, and the plates were then brought back to the fume hood and the lipid classes were identified by comparing with known standards (Sigma Chemical Co.). The marked areas corresponding to the PL fraction was scraped and transferred to glass tubes and dissolved in Arvidson’s solution. The tubes were then capped and mixed using a vortex mixer, frozen overnight at −40°C and then trans-methylated.

The fatty acid composition of the separated lipid group was analysed using the method described by Mason and Waller^{(Reference Mason and Waller35)}. Extracts were trans-methylated overnight using 2′,2′-dimethoxypropane, methanolic HCl and benzene at room temperature. For cells, fatty acid methyl esters were prepared by adding hexane + 0·1 % BHT (1 ml) to the reaction tubes followed by a solution of saturated NaHCO₃ (2 ml). The organic layer was transferred to glass tubes and evaporated at 60°C under N₂ gas. The residues were redissolved in hexane + 0·1 % BHT (50 µl) and transferred to GC vials.

The total fatty acid composition of the PL fraction from the skin tissue and total fatty acids from the cells were determined as follows. Methyl esters were separated and analysed in a GC (Hewlett Packard 6890; HP) with a split injector using an SGE BPX70 capillary column (length, 60 m; internal diameter, 0·25 mm; and film thickness, 0·25 μm; SGE Analytical Science), flame ionisation detector and HP Chem Station software. He was used as the carrier gas, and both the injector and detector temperatures were 280°C. The oven temperature started at 50°C for 1·2 min and was then increased to 170°C at a rate of 4°C/min, then to 200°C at a rate of 0·5°C/min, and finally to 280°C at a rate of 10°C/min. The individual fatty acid peaks were identified by comparing the retention times with validated standards; GLC reference 463 and 85 (Nu-chek Prep). The absolute amount of fatty acid per gram of tissue or cells was calculated using 23:0 methyl ester as an internal standard (IS). Unidentified peaks were not included in the total fatty acid calculation.

The VLC-PUFA composition of the cells was analysed using a Scion 436-GC with a split/splitless injector (splitless 1 min) with a Restek Rxi-5ms capillary column (length, 30 m; internal diameter, 0·25 mm; and film thickness, 0·25 mM), flame ionisation detector and CompasCDS Software. Hydrogen was used as the carrier gas, with split injection and detector temperatures of 250°C and 270°C, respectively. The oven temperature started at 90°C for 1·0 min and was ramped up to 200°C at a rate of 45°C/min, then to 280°C at a rate of 2·5°C/min, and finally to 340°C at a rate of 10°C/min. Data were calculated by comparing the area peaks to the known amount of 23:0 IS added to the samples and presented as area percentage of the selected fatty acids.

Gene expression analysis

Fibroblasts were harvested for gene expression analysis immediately after creating the scratch (0 HPS) in the scratch assay (n 6 for all groups), and 1 d post-scratching (1 DPS; n 6 for the VLC-Conc2 and DHA groups, n 9 for the control group). In brief, wells were washed once in PBS before being lysed using RNeasy lysis buffer. A sterile cell scraper with a two-position blade (Starstedt) was used to loosen the cells, which were then transferred to QIAshredder spin columns, centrifuged at 550 × g for 5 min and stored at –80°C for later analysis.

Total RNA was isolated from fibroblasts using RNeasy Plus Mini Kit (Qiagen) according to the manufacturer’s protocol. All samples were treated with DNase I (Invitrogen) to remove genomic DNA. The concentration and purity of RNA were evaluated using a NanoDrop 1000 Spectrophotometer (NanoDrop Technologies). cDNA was synthesised from 725 ng of RNA in a 20-μl reaction volume using Taqman RT reagents (Applied Biosystems) under the following conditions: 25°C for 10 min, 37°C for 30 min to synthesise cDNA and 95°C for 5 min to terminate the cDNA synthesis reaction. The quantitative PCR reaction mixture consisted of 4 μl of diluted (1:10) cDNA, 1 μl of forward and reverse primers (final concentration of 0·5 μM) and 5 μl of PowerUp SYBR Green Master Mix (Applied Biosystems). A standard curve was included for each primer pair to evaluate the primer efficiency. All the primers used are listed in Table 4. All samples were analysed in parallel, and non-template and non-enzyme controls were included. The quantitative PCR reaction was run on a QuantStudio 5 instrument (Thermo-Fisher Scientific) under the following conditions: initial denaturation, 95°C for 20 s; amplification, 40 cycles at 95°C for 1 s and 60°C for 20 s; melting, 95°C for 1 s and 60°C for 20 s; dissociation, 95°C for 1 s. EF1A, RPOL2 and GAPDH were evaluated as reference genes using RefFinder^{(Reference Xie, Xiao and Chen36)} to identify which was most stable. The relative gene expression level was calculated according to the DDCt method with efficiency correction (Pfaffl 2004) using RPOL2 as a reference gene^{(Reference Pfaffl37)}.

Table 4. Primers used for quantitative PCR analysis of human dermal fibroblast genes

Statistical analysis

Data are expressed as mean ± standard error of the mean (sem) or pooled sem. For the salmon feeding trial, weights and growth data were collected from three replicate tanks with 100 individual fish in each. Growth rates were calculated based on average fish weight in each tank. Tank values were used as experimental units (n 3). Ten fish per tank, giving a total of thirty fish per dietary group, were collected for fatty acid composition analysis. Tank values were used as experimental units (n 3), and linear regression models were used to evaluate the relationship between fatty acid tissue content and n-3 VLC-PUFA levels in the feed. For histology, five fish from each tank, giving a total of fifteen fish per treatment, were analysed. For the salmon keratocyte migration trial, data were collected from a total of six individual fish in the control group, seven in the FGF group, and five for each of the 10 uM VLC-PUFA and 20 uM VLC-PUFA groups. The individual fish were used as experimental units. For each fish, the number of scales with cell migration was divided by the number of attached scales (varying from 3–10 scales), and the mean of all wells for each fish was used in the calculations. For the human dermal fibroblast scratch assay trial, three separate trials were used, with separate thawing of the cell batch for each trial, where each test group includes 6–9 individual wells. Data are presented as mean ± sem of each trial, where n 3. Data for the human dermal fibroblasts gene expression analysis were collected from two separate scratch assay trials: one for the 0 HPS (n 6 in all groups) and another for the 1 DPS (n 6 in DHA and VLC-Conc2 groups, and n 9 in control group), where the experimental unit represents individual wells. One-way ANOVA was used to assess differences between the groups, and significant (P < 0·05) differences were ranked according to Tukey’s honest significant difference test. JMP Pro 13.1.0 (SAS Institute Inc., 1989–2019) and Microsoft Office Excel software were used for the statistical analyses, and GraphPad Prism 9.3.0 was used to create the figures.