Feed ingredients and experimental diet

Two maize types, Bt-maize (MON810) and its near-isogenic maternal line (non-GM (nGM) maize), were derived from planted seed varieties PR34N44 and PR34N43, respectively, provided by Pioneer. They were grown simultaneously in neighbouring fields in Spain. All the maize grains were dried and ground just prior to diet preparation to obtain whole-maize meal. Feeds were prepared by Nofima AS. Diet formulations are given in Table 1. Yttrium oxide was added as a biological marker for apparent digestibility determinations. All diets were balanced regarding vitamins and minerals according to estimated requirements⁽¹⁸⁾. Protein, lipid and energy levels were kept as similar as possible and were comparable between each nGM diet and GM counterpart with and without SBM, respectively. The diets were extruded with a feed particle (pellet) size of 3·5 mm. Salmon feed production using extrusion is a common practice in Norwegian aquaculture. Rausell et al. ⁽Reference Rausell, Pardo-López and Sánchez¹⁹⁾ reported that heat up to 60°C did not denature the pore-forming domain of the Cry1Ab protein, although the receptor-recognising domains may be more heat sensitive, and Xu et al. ⁽Reference Xu, Cao and He⁵⁾ reported anti-Cry1Ab binding to Cry1Ab protein treated at 100°C for up to 60 min. Hence, Cry1Ab protein integrity is expected to be at least partially intact following extrusion.

Table 1 Formulation and proximate composition of the experimental diets on an as-fed basis

nGM, non-GM; Bt, Bacillus thuringiensis; SBM, soyabean meal.

* Residue = DM–(protein+lipids+starch+ash).

† Gross energy was calculated using the energy concentrations of 39·5 for lipid, 23·6 for protein and 17·2 kJ/g for starch.

Experimental design and facilities

The experiment was carried out using a 2 × 2 factorial design with four diet groups. The factors GM and SBM inclusion were tested separately and in combination. The feeding trial was conducted at the aquaculture research facilities of Nofima AS following the institutional and national guidelines for the care and use of animals, and approved by the National Animal Research Authority in Norway. Post-smolt Atlantic salmon of the Sunndalsøra breed with an initial average weight of 93·8 (se 0·3) g were randomly allocated, 100 fish per tank, to twelve tanks. Triplicate tanks of fish were fed one of the four experimental diets. Water surface area in the tanks was 1 m² and water depth 50 cm. The tanks contained filtered running seawater with a temperature of 8·0 ± 0·5°C and salinity between 31 and 32‰. Fish were continuously fed by automatic disc feeders. During the trial, fish were subjected to a 24 h light photoperiod.

Sampling

Sampling was conducted following 33 and 97 d of dietary exposure to the experimental diets. The fish were not fasted before the samplings, as this reduces potential diet-induced inflammatory changes in the intestine⁽Reference Baeverfjord and Krogdahl¹⁵⁾ as well as changes in physiological parameters⁽Reference Krogdahl and Bakke-McKellep²⁰⁾. A total of ten randomly selected fish per tank were anaesthetised, individually weighed and body (fork) length measured. Blood was collected from the caudal vein by means of a heparinised medical syringe. Organs including liver, spleen, head kidney, gonads (the latter only large enough to be weighed at 97 d) and the different regions of the intestine were removed and weighed for calculation of organosomatic indices. Prior to weighing, the intestinal tract was cleared of visceral fat and luminal content, and then divided into proximal intestine (PI), mid intestine (MI) and DI, as described earlier⁽Reference Nordrum, Krogdahl and Røsjø²¹⁾. From four of the ten fish per tank, samples from the PI, MI, DI, spleen, head kidney and liver for histological examination were collected, fixed in 4 % buffered formaldehyde solution for 24 h and subsequently stored in 70 % ethanol until further processing. For mRNA expression investigations, DI tissue samples were rinsed in sterile PBS, transferred to RNA later for 24 h and stored at − 20°C. Head kidney, spleen and intestinal samples for protein expression and/or digestive enzyme analyses were frozen in liquid N₂ and stored at − 80°C. Intestinal contents of MI (at 97 d only) and DI (at both 33 and 97 d) were gathered from ten fish, weighed and freeze-dried. Faeces were collected from thirty fish by stripping from the DI, pooled and frozen on dry ice for digestibility measurements. For composition analyses, whole fish and livers from an additional five fish per tank at the 97 d sampling time were pooled, frozen in liquid N₂ and stored at − 80°C.

Chemical composition analyses

Diets and faeces were analysed for DM, crude protein, crude lipid, starch, ash (mineral) and yttrium oxide (Y₂O₃), the latter by inductivity coupled plasma mass spectroscopy, as previously described⁽Reference Refstie, Helland and Storebakken²²⁾. Whole fish and livers were analysed for DM, crude protein and crude lipid. Liver glycogen was also analysed. DM was measured by drying at 103°C for 24 h with the exception of faeces, which were freeze-dried. For ash, samples were weighed before and after burning at 540°C. Fat in liver and whole body was determined gravimetrically after ethyl-acetate extraction and the fat in feed and faeces after acid hydrolysis and extraction with diethyl ether. N was measured with a nitrogen determinator (LECO FP-428; Väsby) according to Association of Official Analytical Chemists (AOAC) official methods of analysis⁽Reference Soderberg and Cunniff²³⁾ and crude protein calculated as N × 6·25. Starch and glycogen were measured by enzymatic degradation⁽Reference Hemre, Lie and Lied²⁴⁾.

Haematology, plasma clinical chemistry and detection of plasma Cry1Ab protein and specific antibodies

Blood smears of whole blood on microscope slides were prepared for differential blood cell counts using standard techniques. Haematocrit was immediately measured using microhaematocrit tubes centrifuged at 13 000 rpm for 5 min. Erythrocyte counts and Hb were measured on a Cell-Dyn 400 (Sequoia-Turner) according to the manufacturer's instructions, using Para 12 control blood (Streck) for calibration.

The rest of the whole blood was centrifuged at 3000 g for 10 min to obtain the plasma fraction. Plasma clinical chemistry was performed at the Central Laboratory of the Norwegian School of Veterinary Science using Advia^® 1650 (Bayer Healthcare), an automated analysis system for clinical chemistry. Total protein, globulins, albumin, alanine aminotransferase, aspartate aminotransferase, alkaline phosphatase, amylase, lipase, TAG, total bilirubin, total bile acids, NEFA and cholesterol were analysed using standard techniques.

Cry1Ab protein levels and specific antibodies in plasma were determined as previously described⁽Reference Walsh, Buzoianu and Gardiner²⁵⁾ and modified for salmon. Briefly, plasma Cry1Ab protein levels were analysed by ‘sandwich’ ELISA using a commercially available kit QuantiPlate for Cry1Ab/Cry1Ac (Envirologix) following manufacturer's instructions. A standard curve was prepared by using purified Cry1Ab protein standards (0–5 μg/ml) provided in the kit. The mean absorbance read at 450 nm against reference wavelength 630 nm was calculated and used to determine sample concentrations. Positive and negative controls were prepared with the kit Cry1Ab-positive control solution as internal standards. The matrix-specific limit of detection of the adapted kit was determined by interpolation at optical density units (ODmatrix) from the Cry1Ab standard curve. ODmatrix units were determined to be 3 sd from the mean of a population of negative samples measured for a specific matrix. The criteria for positive samples was to exceed the matrix-specific limit of detection.

For detection of specific antibodies against Cry1Ab in plasma, ELISA plates were coated overnight at 4°C with 1 mg/ml of purified Cry1Ab toxin (a fermentation product of B. thuringiensis var. Kurstaki from Dipel, produced by Valent BioSciences Corporation) in 0·05 m-carbonate–bicarbonate buffer (pH 9·6). The plates were blocked for 1 h at 37°C with 0·01 m-PBS (pH 7·4), containing 1 % gelatine. PBS alone or serial dilutions (from 1:5 to 1:78 125) of fish plasma were added to the plates and incubated for 1 h at 37°C. Plates were then incubated with anti-fish IgM mouse IgG1 (1:16 000) antibodies for 1 h at 37°C. Following this, biotin-labelled anti-mouse IgG1 antibody conjugate (1:5000) was added to the wells and the plates were incubated for 1 h at 37°C. Horse-radish peroxidise-labelled avidin conjugate was subsequently added and the incubation step was repeated. For colour development, H₂O₂/o-phenylenediamine-containing substrate solution (pH 5) was added and the plates were developed for 5 min in the dark. The enzyme reaction was stopped by the addition of 4 m-H₂SO₄. The absorbance was read at 492/630 nm. Samples were analysed in duplicate and the washing procedure repeated after each step involved manually washing the plates twice with PBS containing 1 % gelatine and decanting. Antibody titre was defined as the maximum serum dilution with an absorbance measurement higher than the blank signal plus three times the standard deviation.

Histology

All formalin-fixed tissues were routinely dehydrated in ethanol, equilibrated in xylene and embedded in paraffin according to standard histological procedures. Sections of 5 μm were stained with haematoxylin and eosin and blindly evaluated under a light microscope. Distal intestinal morphology was scored according to the criteria previously described in Atlantic salmon with SBM-induced enteritis⁽Reference Baeverfjord and Krogdahl¹⁵⁾: (1) widening and shortening of the intestinal folds; (2) loss of the supranuclear vacuolisation in the absorptive cells (enterocytes) in the intestinal epithelium; and (3) cellular infiltration of a mixed leucocyte population in the central lamina propria within the intestinal folds as well as in the submucosa. The degree of histological changes was assessed as normal, mild, moderate or severe.

Digestive enzyme activities and bile acid concentrations

Leucine aminopeptidase activity in the PI, MI and DI tissue was analysed to assess intestinal function following the method described previously⁽Reference Krogdahl, Bakke-McKellep and Baeverfjord²⁶⁾. Activities are related to mmol substrate hydrolysed per unit time in the whole tissue per kg body weight (enzymatic capacity) and per mg protein (specific activity). Protein was analysed using the Bio-Rad Protein Assay (Bio-Rad Laboratories).

For trypsin activity analysis, 50 mg freeze-dried intestinal content was homogenised and suspended in 2 ml dH₂O. Trypsin activity was measured colorimetrically according to Kakade et al. ⁽Reference Kakade, Hoffa and Liener²⁷⁾, using the substrate benzoyl-arginine-p-nitroanilide (Sigma-Aldrich). The trypsin activity is expressed as the change in optical density units (U) and related to mg DM. The bile acid concentrations in the intestinal contents were analysed using the Enzabile^® kit from Nycomed Pharma AS Diagnostics.

Quantitative real-time PCR

RNA purification and quality control, DNase treatment, complementary DNA synthesis, primer optimisation and quantitative PCR assays were performed as described in detail elsewhere⁽Reference Kortner, Valen and Kortner²⁸⁾. Quantitative PCR primers were obtained from the literature or designed using Primer3 software (http://frodo.wi.mit.edu/primer3). See Table 2 for details. β-Actin (ACTB), RNA polymerase II (RNAPOLII), hypoxanthine phosphoribosyltransferase 1 (HPRT1) and glyceraldehyde-3-phosphate dehydrogenase (GAPDH) were evaluated for use as reference genes by ranking relative gene expression according to their stability, as described previously⁽Reference Kortner, Valen and Kortner²⁸⁾. A combination of GAPDH and RNAPOLII was used as normalisation factor. Distal intestinal mean normalised expression of the target genes was calculated from raw C _q values using a plate calibrator-normalised relative quantification⁽Reference Muller, Janovjak and Miserez²⁹⁾.

Table 2 Primer pair sequences, amplicon size (AS), annealing temperature (AT), efficiency (E) and Genbank accession number for genes used for quantitative real-time PCR

CD4, cluster of differentiation 4; TGF-β, transforming growth factor β; IFN-γ, interferon-γ; PCNA, proliferating cell nuclear antigen; HSP70, heat shock protein 70; CAT, catalase; SOD, superoxide dismutase; PEPT, peptide transporter; SGLT, sodium-dependent glucose transporter; ACTB, β-actin; RNA-POLII, RNA polymerase II; HPRT1, hypoxanthine phosphoribosyltransferase 1; GAPDH, glyceraldehyde-3-phosphate dehydrogenase.

Western blot analysis

A measure of 50 mg tissues samples from DI, head kidney and spleen were homogenised with 400 μl cold radioimmunoprecipitation assay lysis buffer (50 mm-Tris–HCl (pH 8·0), 150 mm-NaCl, 0·1 % SDS, 1 % Igepal CA-630, 0·5 % sodium deoxycholate, 2·5 mm-phenylmethylsulfonyl fluoride (PMSF), 2·5 mm-EGTA, 4 mm-ethylene glycol tetraacetic acid (EGTA), 5 mm-sodium orthovanadate, 5 μg/ml aprotinin, 50 μg/ml leupeptin, 2 μg/ml pepstatin, 0·2 mg/ml benzamidine and 10 mm-sodium fluoride). The homogenates were centrifuged at 16 000 g at 4°C for 20 min and supernatants were collected. Protein content was quantified using the Bradford assay (Bio-Rad) with bovine serum albumin (BSA) as a standard.

Samples of 10 μg protein were prepared for SDS-PAGE and transferred to a nitrocellulose membrane (Invitrogen). Membranes were incubated with primary antibodies: rabbit polyclonal anti-GAPDH (1:250; Abcam); mouse monoclonal anti-CD4 (1:50; provided by Karsten Skjødt, University of Southern Denmark); and mouse monoclonal anti-proliferating cell nuclear antigen (PCNA) (1:2000; Dako) in 1 ×  Tris-buffered saline with Tween-20 (TBST) (50 mm-Tris–HCl (pH 7·5), 150 mm-NaCl, 0·1 % Tween 20) with 5 % non-fat dry milk and subsequently incubated with the alkaline phosphatase-conjugated secondary antibodies. The targeted proteins were visualised with fluorescence by ECF™ Western Blotting reagent Pack (GE Healthcare) and Typhoon 9200 imager system (Amersham Biosciences). ImageQuant software (Amersham Biosciences) was applied to quantify the band intensities. GAPDH was used as a reference for normalisation of the target protein expressions.

Calculations

$$\begin{eqnarray} Condition\,factor\,( K ) = (body\,weight/fork\,length^{3})\times 100. \end{eqnarray}$$

$$\begin{eqnarray} Organosomatic\,index = (organ\,weight/body\,weight)\times 100. \end{eqnarray}$$

$$\begin{eqnarray} Specific\,growth\,rate = ((ln\,final\,weight - ln\,initial\,weight)\times 100)/ t ;\, t = time\,in\,d. \end{eqnarray}$$

$$\begin{eqnarray} Feed\,efficiency = weight\,gain\,(g)/feed\,intake\,(g). \end{eqnarray}$$

$$\begin{eqnarray} Apparent\,digestibility\,coefficient\,(\%) = 100 - (100\times (nutrient\,in\,faeces/yttrium\,oxide\,in\,faeces)\times (yttrium\,oxide\,in\,feed/nutrient\,in\,feed)). \end{eqnarray}$$

$$\begin{eqnarray} Nutrient\,retention\,efficiency = 100\times nutrient\,gain/nutrient\,intake. \end{eqnarray}$$

$$\begin{eqnarray} Mean\,corpuscular\,volume = (haematocrit/erythrocytes)\times 10. \end{eqnarray}$$

$$\begin{eqnarray} Mean\,corpuscular\,Hb = (Hb/erythrocytes)\times 10;\,Hb = Hb\,(g/100\hairsp ml). \end{eqnarray}$$

$$\begin{eqnarray} Mean\,corpuscular\,Hb\,concentration = (Hb/haematocrit)\times 100. \end{eqnarray}$$

Statistics

The data were statistically evaluated using JMP version 9.0 (2010) Statistical Discovery™ (SAS Institute, Inc.). Normal distribution of data was tested using a plot of actual v. predicted residuals and the Shapiro–Wilk W-statistic on the residuals. The results were subjected to two-way ANOVA, with GM and SBM inclusion as the class variables. The data for mRNA expression (n 7 or 8) and protein levels (n 3) were analysed based on individual fish, while for other data tank means (n 3) were used. For the histological evaluation, results were compared using the χ² test. All reported P values are two-sided and significance was set at P< 0·05.