Diets

Four similar diets with high content of plant ingredients, deficient choline level, and varying in lipid level from 16, 20, 25 and 28 % were formulated. The diets were formulated to be iso-nitrogenous, as often recommended for nutritional studies. This means that with increasing lipid content in the diet, ingredients with low protein content had to be replaced with ingredients with a higher protein level. For each step up of lipid in the diet, the alteration in these plant ingredients were changed proportionally, i.e. increasing level of maize gluten (80 % protein) and decreasing a mixture of SPC and wheat, all of high quality. The variations were expected not to change nutrient digestibility or passage rate. The formulations and macronutrient compositions are shown in Tables 1a and 1b. The diets were supplemented with standard vitamin and mineral premixes in accordance with NRC guidelines (2011)⁽²³⁾. Yttrium oxide (0⋅50 g/kg) was added as an inert marker for estimation of apparent nutrient digestibility. The diets were formulated to contain level of long-chain ω3 fatty acids well above requirements to avoid other causes of steatosis than choline deficiency. The experimental diets were produced by extrusion (feed pellet size 6 mm) using a BC 45 twin screw extruder (Clextral, France). Upon arrival of the diets at the experimental site, fat leakage from the diet with 28 % fat was discovered. A new diet was made with higher content of soy lecithin for better emulsification. The consequences of the intervention, i.e. a dietary choline level higher than planned, was not realised until after the feeding period was completed. However, this unexpected event was found not to significantly disturb the aims of the experiment. Even though the results obtained for the diets containing 16, 20 and 25 % of lipid level were sufficient to draw conclusions regarding the aims of the study, the results for the 28 % diets are included in this presentation. In fact, the higher choline level in the 28 % lipid diet supplied useful additional information, confirming not only that the severity of the steatosis in the pyloric caeca varies with choline supply, but also the important role of choline for sufficient lipid transport and metabolism in the pyloric caeca. Additionally, to include the results for the diet with 28 % lipid, also strengthens the statistical power of the experiment.

Table 1a.

Diet receipts and results and nutrient content as formulated and analysed

* See materials and methods for explanation and considerations regarding the high choline level in the D28 diet.

Table 1b.

Content of fatty acids in the diets, % of sum of fatty acids*

MUFA,  monousaturated fatty acids.

* The results show the area of peak for the fatty acid in the chromatogram given as % of sum of the fatty acids areas of which some were not identified.

Experimental animals and conditions

The feeding trial was conducted at Nofima's Research Station in Sunndalsøra (NO), which is approved by Norwegian Animal Research Authority (NARA) and operates in accordance with Norwegian Regulations of 17th of June 2008 No. 822: Regulations relating to Operation of Aquaculture Establishments (Aquaculture Operation Regulations). Trial fish were treated in accordance with the Aquaculture Operation Regulations during the experiment. As no harmful procedures were forced upon the fish before euthanisation, a specific permission was not needed for this experiment. Atlantic salmon with an average initial weight of 24 g were assigned to 0⋅6 × 0⋅6 m² (125 L) flow through tanks, 140 fish per tank. Each diet was fed to fish in duplicate tanks for each dietary treatment, and each water temperature: 8 and 15 °C, i.e. a total of sixteen tanks. The temperature range is considered to cover the optimal range for Atlantic salmon^{(Reference Falconer, Hjøllo and Telfer30)}. A 24 h light regime was employed. Water temperature was measured daily, and dissolved oxygen weekly to secure 80–100 % of saturation. To secure feeding to satiation, the fish were fed 15 % in surplus of anticipated requirement, according to feeding tables and expected growth rate, using belt feeders.

Sampling

After 5 weeks of feeding, the biomass in each tank was reduced to keep biomass at a lower level to ensure sufficient oxygen supply. A total of fifty fish were randomly removed from each tank at the highest temperature, and twenty fish per tank at the lower temperature, to similar biomasses in all tanks. After another 3 weeks of feeding, six fish in fed state from each tank were sampled randomly, anaesthetised with tricaine methane-sulfonate (MS-222) and killed by a sharp blow to the head, in accordance with the Norwegian Animal Welfare act. Weight and length of each sampled fish were recorded. Fish remaining in the tanks at the end of the sampling were weighed in bulk. Total weight gain was calculated by adding up the weights of the sampled and the remaining fish. Blood was sampled from the caudal vein into vacutainers with lithium heparin and kept on ice. After centrifugation, plasma was collected in 2 ml aliquots, frozen in liquid nitrogen and kept at 80 °C. Following blood sampling, the fish were opened ventrally, and the abdominal organ package was removed from the abdominal cavity. The liver was separated from the package and weighed. Thereafter, the intestine, freed of external fat was sectioned as follows: PI, the section from the pyloric sphincter to the most distal pyloric caecum; mid intestine (MI), from the latter pyloric caecum to the earliest area with higher diameter and darker pigmentation, distal intestine (DI), from the latter end of the MI to the anus. The sections were opened and digesta from the section were collected, snap-frozen in liquid N₂ and stored at −80 °C. Those fish found with empty intestine were excluded from the sampling. Each intestinal section was then weighed before tissue samples were collected for histological and gene expression analyses. The samples for histological examination were immediately fixed in 10 % neutral-buffered formalin (4 % formaldehyde) and kept at room temperature. Whereas the samples for gene expression analyses were rinsed in sterile saline water, stored in RNA later® at 4 °C, and moved to −40 °C after 24 h. The fish that were removed for reduction of biomass at 5 weeks were stripped for faeces, while the remaining fish in the tanks were stripped for faeces at termination of the experiment, method as described by Austreng^{(Reference Austreng31)}. The faecal samples were pooled for each tanks, frozen in liquid N₂ and stored at −20 °C.

Chemical analyses of feed, gut contents, plasma, PI and liver including fatty acid analyses (FAME)

Samples of the feed and faeces were analysed for dry matter (DM), ash, crude protein (CP) and crude fat (CF) and energy at Nofima, Sunndalsøra. Fatty acid content was analysed at the Department of Animal and Aquacultural Sciences, Norwegian University of Life Sciences, Ås, Norway. DM was determined by drying the samples to a constant weight at 103 °C. Determination of ash content, samples were combusted at 550 °C for 10 h. Total nitrogen was analysed by Kjeldahl auto analyzer, and energy by bomb calorimetry (Parr 1271 adiabatic bomb calorimeter). Fatty acid composition was quantified by the FAME method described by O'fallon^{(Reference O'Fallon, Busboom and Nelson32)}. Choline level in the diets was analysed by Eurofins. The method involves extraction by methanol and water, alkaline hydrolysis to free choline from phosphatidyl choline, and quantification by isotope dilution LC-MSMS. The choline results show total choline, free and bound.

Analyses of yttrium content in feed and faeces were carried out by pre-digestion with concentrated ultrapure HNO₃ at 250 °C using a Milestone microwave UltraClave III (Milestone Srl, Sorisole, Italy). Samples were then diluted (to 10 % HNO₃ concentration), and yttrium was determined by inductively coupled plasma optical emission spectrometry (ICP-OES analysis) with a PerkinElmer Optima 5300 DV (PerkinElmer Inc., Shelton, CT, USA). The plasma nutrient and cholesterol analyses were carried out at the Central Lab of the Faculty of Veterinary Medicine, by standard hospital methods.

Histology

Pyloric caeca samples were processed at the Norwegian University of Life Sciences (NMBU) using standard histological techniques: dehydration in graded ethanol, clarification in xylene, embedding in paraffin and sectioning of 5 μm thick sections. The sections were then dewaxed, re-hydrated and stained with haematoxylin and eosin to perform the histological evaluation. The samples were randomised, and the main signs of vacuolation were assessed using a light microscope. According to the proportion of tissue affected by the presence of lipid-like vacuoles, swollen and irregular cells and condensed nuclei, the severity of the syndrome was scored as Normal (≤10 %), Mild (10–25 %), Moderate (25–50 %), Marked (≥50 %) and Severe (≥75 %) (Fig. 1).

Figure 1.

Histological severity of vacuolation of the pyloric caeca tissue (steatosis) representative for (a) normal, (b) moderate, (c) marked and (d) severe.

RNA extraction, cDNA synthesis and gene expression analyses

Gene expression analysis was performed from ninety-six samples collected from the pyloric caeca of the same six fish per tank used for the preceding analyses. Gene expression profiling was conducted by Quantitative Real-Time PCR (qPCR) following the MIQE guidelines^{(Reference Bustin, Benes and Garson33)}. Total RNA was extracted from pyloric caeca samples (around 30 mg) using a Ultraturrax homogenizer, TRIzol® reagent (Invitrogen, ThermoFisher Scientific) and chloroform according to the manufacturer's protocol. Obtained RNA was DNase treated (TURBO™, Ambion, ThermoFisher Scientific) and purified with PureLink RNA mini kit (Invitrogen, ThermoFisher Scientific). RNA purity and yield was measured using a NanoDrop ND-1000 Spectrophotometer (NanoDrop Technologies) and RNA integrity was assessed by 2100 Bioanalyzer by the use of a RNA Nano Chip (Agilent Technologies). Total RNA was stored at −80 °C for upcoming analyses. Before proceeding with the synthesis of the first-strand cDNA, the RNA from the fish of each tank was pooled two by two. Afterward, 0⋅8 μg of the total pooled RNA, oligo (dT)₂₀ primers and Superscript III in 20 μl reactions (Invitrogen) were used to conduct the synthesis. To achieve negative controls, the same process was performed, omitting RNA and enzyme. cDNA was then diluted 1:10 and stored at −20 °C before the following qPCR procedure. The gene expression profiling was performed on a pool target genes involved in lipid metabolism, lipid uptake and transport and phosphatidylcholine synthesis. The primers to be used in the qPCR reaction were obtained from literature and from previous works conducted in this group^{(Reference Hansen, Kortner and Krasnov9,Reference Hansen, Kortner and Denstadli12)} . Additional information concerning genes name or primers source, efficiency and size, is shown in Supplementary Table S1. For new assays, primer optimisation was carried out by PCR gradient assays, followed by assessment of PCR reaction efficiency (E) using serial dilutions of a pool of randomly selected cDNA samples. A LightCycler 96 (Roche Diagnostic) was used to perform DNA amplification and gene expression analyses. Each reaction mix contained 2 μl PCR-graded water, 5 μl of LightCycler 480 SYBR Green I Master mix (Roche Diagnostics) and 0⋅5 μl of both forward and reverse primer. Every sample was analysed in duplicate alongside a no template control. The three-step qPCR program included an enzyme activation step at 95 degrees for 5 min, followed by 40–45 cycles of 95 degrees (10 s), 55, 58, 60 or 63 °C (10 s), and 72 °C (15 s). Quantification cycle (Cq) values were calculated using the second derivative method. The products obtained from the qPCR were assessed analysing the melting curve. To perform relative normalisation of the qPCR assay, a pool of reference genes was selected as suggested by Kortner et al. ^{(Reference Kortner, Valen and Kortner34)}. Considering the absence of a universally stable reference gene, we tested the stability of a selected pool already used by our group for several previous studies conducted on the pyloric caeca of Atlantic salmon^{(Reference Hansen, Kortner and Krasnov9,Reference Krogdahl, Hansen and Kortner11)} . The most stable reference genes, selected based on their overall coefficient of variation (CV) and their interspecific variance were RNA polymerase II (rnapoli), hypoxanthine phosphoribosyl transferase 1 (hprt1) and glyceraldehyde-3-phosphate dehydrogenase (gapdh). Mean normalised expression of the target genes was calculated from raw Cq values by relative quantification^{(Reference Muller, Janovjak and Miserez35)}. The panel of target genes was the same used by Hansen et al. ^{(Reference Ballester-Lozano, Benedito-Palos and Estensoro8–Reference Hansen, Kortner and Denstadli10)} and it is represented by a set of genes involved in lipoprotein assembly, choline and phosphatidylcholine synthesis and cholesterol synthesis. As also done in the previously cited studies by Hansen et al., among the whole pool of genes, four were selected as main molecular biomarkers because of their particular receptiveness to steatosis: plin2, apoA-I, apoA-IV and pcyt1α.

Calculations

Fish growth was calculated as specific growth rate (SGR, percentage growth per day)= ((ln FBWg/ln IBWg)/D) × 100. IBW and FBW represent the initial and final body weight as tank means, and D represents the number of feeding days. The condition factor was calculated as: CF =((FBW × 100)/fork length cm³). The organosomatic indices (OSI) were calculated as: (organ weight g/body weight g) × 100. Apparent digestibility (AD) for each nutrient was determined by using yttrium oxide (Y₂O₃) as inactive marker and estimated as follows: AD_n=100 – (100 × (M _feed/M _faeces) × (N _feed/N _faeces)), where M represents the percentage of Yttrium oxide in feed and faeces and N represents the percentage of a specific nutrient in feed and faeces.

Statistical analyses

In light of the fact that this experiment was a screening study and had a regression design with close relationship between the five treatments, duplicate observations were considered sufficient. The design gives 11 degrees of freedom for the error term, and a reasonably accurate estimate of the error. Tank mean was used as the statistical unit. The results were subject to two-way analyses of variance (ANOVA) with lipid level and temperature as class variables. The Shapiro–Wilk test was used to assess the normality of the variance. The Tukey's test was used rank treatments in the molecular analyses, while Duncan's test was used for the other results. The level of significance for all analyses was set at P < 0⋅05, and P-values between 0⋅05 and 0⋅1 were considered to indicate a trend in effects as indicated in the text. The plan was to evaluate the results by regression analyses, but the event described above in the production of the D28 diet, made the result for the diet with the highest lipid content unsuitable for regression analyses. The two-way ANOVA was therefore chosen as the most suitable method.