Potential health and environmental risks of GM crops are still being debated about in Norway and other European countries. Some uncertainty is linked to the ingestion of GM plants modified to express insecticidal Bt (Bacillus thuringiensis) toxins, also known as Cry proteins, due to their potential adjuvant properties(1). These proteins are naturally produced by the spore-forming soil bacterium B. thuringiensis. In targeted insects, the different Cry proteins bind to specific receptors in the mid-intestine and cause damage to the intestinal wall by forming pores, thus changing the permeability of epithelial cells and eventually resulting in death(Reference Knowles2). The Norwegian Scientific Committee for Food Safety has questioned the safety of Bt-toxins and identified knowledge gaps(3). It may be premature to accept that the detrimental effects are limited to the targeted organisms only(Reference Then4). The first line of defence when an organism is exposed to a potential toxicant via feed is the barrier of the intestinal tract. In the present study, we measured several intestinal biomarkers at the gene transcript level including a thorough histological evaluation. The gene transcripts covered important cellular pathways and intestinal functions including gene transcripts linked to the digestion of starch and absorption of glucose, appetite control, cellular DNA repair, oxidative stress and apoptosis. To further investigate possible mechanisms of effects, global DNA methylation was investigated in embryos. It was hypothesised that the crystal protein 1Ab (Cry1Ab) protein or other factors in Bt-maize could affect the methylation either directly or indirectly by inhibition of nutrient uptake.
MON810 is one of several modification events producing Bt-maize and has a gene introduced encoding the Cry1Ab protein(Reference Sanders, Lee, Groth and Thomas5). Numerous studies have investigated Bt-maize in terrestrial animal feeds, but few studies have focused on Bt-maize as an ingredient in fish feeds. A recent review has summarised results from fish feeding trials with GM products, including Bt-maize(Reference Sissener, Sanden and Krogdahl6). Increased feed consumption resulting in increased growth has been observed in a short-term feeding study with zebrafish fed Bt-maize(Reference Sissener, Johannessen and Hevroy7). On the other hand, Atlantic salmon post-smolt fed Bt-maize at 15 and 30 % of the total diet exhibited significantly reduced feed intake, growth rate and final weight than those fed non-Bt-maize (near-isogenic line)(Reference Hemre, Sagstad and Bakke-Mckellep8, Reference Sagstad, Sanden and Haugland9), as well as indications of stress and immune responses(Reference Sagstad, Sanden and Haugland9). However, a recent Atlantic salmon study has not confirmed the earlier results of reduced growth(Reference Bakke, Gu and Krogdahl10).
A long-term study with Atlantic salmon fed 12 % Bt-maize has not revealed obvious pathological effects, but indicated changes in plasma TAG levels, intestinal cell proliferation and intestinal glucose uptake(Reference Sanden, Berntssen and Krogdahl11, Reference Sanden, Krogdahl and Bakke-Mckellep12). Thus, uncertainties still remain regarding the safety of MON810 maize in diets used for cultivated fish. Confounding factors in the two maize types used in fish feeds, such as varying levels of mycotoxins(Reference Sissener, Lall and Sagstad13), may be a source of the inconsistent findings between feeding trials using the same Bt-maize event. When measured in the above-mentioned feeding trials, including in the present trials, differences in mycotoxin types (deoxynivalenol (DON), fumonisin B1 (FB1) and aflatoxin B1 (AFLB1)) were observed. Information on the absorption and toxicokinetics of mycotoxins in farmed finfish species is limited, and little or no information is available on the carry-over of dietary mycotoxins from the feed to fish. Limited amounts of data exist on its potential effect on the methylation of DNA(Reference Sanden, Jorgensen and Hemre14). The European Food Safety Authority (EFSA) has made an evaluation of DON as a contaminant in animal feeds, but concluded that no safe level could be established based on the available database (EFSA 2004). Although there is no general consensus on how and when feeding trials should be performed in safety assessments of GM plants(Reference Knudsen and Poulsen15), longer-term studies and generational studies are recommended, particularly where the mode of action of the novel protein or possible unintended effects of the genetic modification are unclear. The EFSA has pointed out that in some cases where the effects of individual substances are not known, longer-term studies with emphasis on reproduction/development should be considered and may be more sensitive than subchronic endpoints(Reference van Haver, Alink and Barlow16). This has been further emphasised in a recent review by Snell et al. (Reference Snell, Bernheim and Bergé17). Longer-term or generational studies are also repeatedly requested by researchers when the effects of GM feeds are identified, but they are struggling to interpret the biological significance due to the limited duration of the studies. Zebrafish has previously been suggested as a model for aquaculture species in the evaluation of GM plant feed ingredients(Reference Sissener, Johannessen and Hevroy7), although it has been recognised that it is less sensitive to certain feed toxicants than, for example, Atlantic salmon and rainbow trout(Reference Sanden, Jorgensen and Hemre14). In the study by Sanden et al. (Reference Sanden, Jorgensen and Hemre14), zebrafish was not found to be an appropriate model when evaluating the effects of contaminated aquaculture feeds on parameters such as growth performance and feed and nutrient utilisation. It may, however, be an adequate aquaculture model when studying the mode of action of various feed ingredients and feed contaminants. In the present study, the generational effects of Bt-maize feeding were investigated. The aim was to investigate (1) the dietary effects of Bt-maize in the parental generation, with a focus on growth and reproductive performance, health parameters and gene transcript biomarkers, and (2) the effects of dietary Bt-maize fed to the parental generation and their offspring, with a focus on one epigenetic marker, larva swimming activity, growth performance and histomorphological evaluation of the intestine, as well as gene transcript biomarkers.
Materials and methods
Diets and feed production
Two casein/gelatin-purified diets were prepared at our laboratory. Table 1 summarises the ingredients used, proximate composition, and mycotoxin and pesticide content. Seeds from maize MON 810 (Bt) and the unmodified parent line (nBt) (PR34N44 and PR34N43, respectively; Pioneer HiBred) were grown simultaneously in neighbouring fields in 2007 in Valtierra, Navarra, Spain. These two maize lines have been thoroughly described by Walsh et al. (Reference Walsh, Buzoianu and Gardiner18) and reported to have only minor differences in proximate and nutrient composition. The preparation of diets involved mixing three different fractions. Gelatin and carophyll pink were dissolved in hot water, at a 9:1 ratio (hot water (about 80°C)–gelatin, w/w), before all the dry ingredients and the oil mixture were carefully added. The blend was mixed in a conventional food processor until becoming homogenous. The paste was poured onto labelled parchment-covered trays and then dried overnight at low temperatures (40°C) in an oven, before grinding, sieving and storing at − 18°C. The same diets were fed to the parental generation (F0) and offspring generation (F1).
nBt, non-Bacillus thuringiensis; Bt, Bacillus thuringiensis; AA, amino acids; DON, deoxynivalenol; NIV, Nivalenol.
* 60 % Dicalcium phosphate dehydrate, 0·01 % cobalt chloride hexahydrate, 0·04 % copper sulphate, 30 % potassium sulphate, 0·1 % potassium iodide, 2 % magnesium sulphate heptahydrate, 0·1 % manganese sulphate, 5·75 % NaCl, 0·01 % sodium selenite, 1 % zinc sulphate heptahydrate, and 1 % iron sulphate heptahydrate.
† 0·1 % Vitamin A, 0·04 % vitamin D3, 2 % vitamin E, 0·1 % vitamin K, 4·3 % vitamin C, 40 % choline, 0·15 % thiamin, 0·19 % riboflavin, 0·2 % pyridoxine, 2 % niacin, 4 % inositol, 0·07 % folic acid, 0·6 % calcium pantothenate, 0·75 % biotin, 0·3 % cobalamin and 45·2 % casein salt.
‡ 4·3 % Taurine, 21·4 % aspartic acid, 6·4 % threonine, 8·5 % glycine, 15·2 % alanine, 4·3 % valine, 5·8 % methionine, 4·3 % isoleucine, 8·5 % leucine, 6·4 % lysine, 8·5 % arginine and 6·4 % tryphtophan.
§ Mycotoxin content in the feed is calculated based on the levels found in the ingredients. Mycotoxins below the detection limit: diacetoxyscirpenol < 10 μg/kg; 3-acetyldeoxynivalenol < 10 μg/kg; 15-acetyldeoxynivalenol < 10 μg/kg; T2 toxin and HT2 toxin < 10 μg/kg; aflatoxin G1 < 0·1 μg/kg; aflatoxin G2 < 0·1 μg/kg.
∥ An array of more than 300 pesticides were analysed in the two diets (Bioforsk), and only diphenylamine was detected above the limit of quantification.
Diet chemical analysis
Moisture in the diets was measured by drying at 103°C for 24 h, ash was weighed after burning at 540°C, and lipid content was measured after extraction with ethyl acetate(Reference Lie and Lambertsen19). N content was measured using a nitrogen determinator (LECO FP-428; LECO Corporation) according to the AOAC (Association of Analytical Communities) official methods of analysis, and crude protein content was calculated as N × 6·25. Starch content was measured by enzymatic degradation as described by Hemre et al. (Reference Hemre, Lie and Lied20). Mycotoxin levels in the experimental diets were analysed by the Norwegian Veterinary Institute by GC–MS(Reference Langseth, Bernhoft and Rundberget21). The content of Cry1Ab in the diets was tested using a commercially available qualitative Bt-Cry1Ab/1Ac ELISA kit (Agdia Biofords). The diets were analysed for pesticide residues by testing against a panel of more than 300 different active substances (BioForsk, Norwegian Institute for Agricultural and Environmental Research, Ås, Norway).
Fish husbandry and experimental design
The trials were conducted in accordance with the Norwegian Animal Welfare Act no. 73 of 20 December 1974 and the Regulation on Animal Experimentation of 15 January 1996. The experiments were run in an AHAB multiple rack zebrafish system (Aquatic habitats, Aquatic Eco-Systems) with reverse osmosis followed by automatic salt dosing of the water, UV, and mechanical and carbon filtration of the water. During the trials, the temperature was 28·5 ± 0·5°C, salinity was 500 ± 30 μS/cm, oxygen was >90 % saturation, photoperiod was 14 h light–10 h dark with lights on from 22.00 to 08.00 hours. Larvae were fed ad libitum with Artemia nauplii for 1 month before starting the parental feeding trial (F0) on 7 February 2011. In this trial, 120 zebrafish larvae (35 d post-hatch, dph) were distributed into six tanks (3·0 litres, n 3) and randomly assigned to one of the following two diets: Bt-maize diet and nBt-maize diet. The offspring feeding trial (F1) was started on 3 October 2011 in which 168 zebrafish larvae (39 dph) obtained from the parental generation (fourth spawning) were distributed into twelve tanks (3·0 litres) and fed one of the following three regimens: Bt-maize diet Bt–Bt (larvae from the Bt-maize diet-fed parental generation, n 4); nBt-maize diet Bt–nBt (larvae from the Bt-maize diet-fed parental generation, n 3); nBt-maize diet nBt–nBt (larvae from the nBt-maize diet-fed parental generation, n 5). Fig. 1 presents an overview of the experimental design. Mortality was recorded on a daily basis. The parental generation feeding trial (F0) followed a restricted feeding regimen, where feeding was adjusted to the growing biomass in each tank and gradually reduced from 10 to 2–3 % of total biomass during the trial. The offspring generation feeding trial (F1) followed a pair-feeding regimen in which the fish tank that demonstrated the lowest feed intake determined the amount of feed offered to the other tanks. Within both the generations, fish in all tanks were given the same amount of feed twice a day and efforts were made to avoid feed waste by giving small portions. Feed particle size was gradually increased with increasing fish size from 315–400 μm up to 560–700 μm at the end of the feeding trial.
Tissue sampling – parental generation
Before handling, all fish were euthanised by immersion in an ice water bath (4°C or less)(Reference Wilson, Bunte and Carty22). After 45 d of feeding, fish were sampled on 24 March 2011 (80 dph). Data on fish performance were recorded from seven to ten randomly selected fish per tank. All fish were wet weighed to the nearest 0·01 g, total length was determined to the nearest millimetre and sex was recorded. Blood was sampled from three to four fish per tank by cutting off the tail posterior to the anal fin and by collecting the blood into capillary tubes coated with heparin. For differential leucocyte counts, a small droplet of blood was placed at the end of a glass slide to produce smears before being fixed in methanol. The mid-intestine was obtained from four fish per tank and dissected using fine surgical tools under magnification before being quickly frozen in liquid N2 and stored for later RNA extraction and gene expression analysis. All remaining fish were pooled into two experimental tanks (10 litres): Bt-maize group: twenty-two fish (two females); nBt-maize group: sixteen fish (four females), and fed the same experimental feeds for another 6 months (1–2 % of the biomass). Fertilised eggs were collected from the Bt-maize and nBt-maize groups on 23 August and larvae that hatched on 25 August (offspring generation). Data on reproductive performance were collected at the following time points in the pooled tanks: at 175–297 dph for fecundity (seven samplings); at 127–183 dph in fertilised eggs for epigenetics (three samplings); at 274–300 dph in F1 larvae for swimming activity (three samplings). Finally, on 16 November 2011, at day 283 (317 dph), all remaining fish from the parental generation (F0) were sampled and wet weighed to the nearest 0·01 g and total length was determined to the nearest millimetre. Livers were collected from ten fish (F0) per diet and dissected before being quickly frozen in liquid N2 and stored at − 80°C for later CuZn superoxide dismutase (SOD) analysis.
Tissue sampling – offspring generation
The offspring larvae were reared in our laboratory under conditions the same as those described for the parental generation. Embryos (51 h post-fertilisation) were collected for global DNA methylation analysis (F1) and larvae (4 dph) were collected for analysing swimming activity (F1). The methodology used is described below. Before the offspring fish sampling (83 dph), which was performed on 16 November 2011, all fish were euthanised by immersion in an ice water bath (4°C or less)(Reference Wilson, Bunte and Carty22). Data on fish performance of all fish were recorded (fourteen fish per tank) using a procedure the same as that used for the parental generation, and the liver and mid-intestine were dissected from six fish as described before, quickly frozen in N2 and stored at − 80°C for later gene expression analysis. For histological evaluation, the whole intestinal tract was immediately sampled and placed into standard Bouin's solution. After fixation, the samples were dehydrated in graded series of alcohol, equilibrated in xylene and embedded in paraffin.
RNA isolation and quantitative real-time RT-PCR (parental generation and offspring generation)
Total RNA was extracted from individual mid-intestinal and liver tissues using the TRIzol reagent according to the manufacturer's instructions (Invitrogen, Life Technologies), and residual genomic DNA was removed by DNase treatment using DNA-free reagents (Ambion). RNA quality and integrity were assessed using NanoDrop ND-1000 Spectrophotometer (NanoDrop Technologies) and the Agilent 2100 Bioanalyzer (Agilent Technologies). A total of twenty-four intestines were sampled from the parental generation (two to three intestines per tank) and seventy-two livers/intestines were sampled from the offspring generation (four livers/intestines per tank). The sequences of the PCR primers used for the quantification of the mRNA transcriptional levels of the target genes as well as the reference genes are given in Table 2 (Invitrogen, Life Technologies). All primer pairs were tested using a one-step RT PCR kit (Qiagen), and the reaction specificity of each assay was verified by observing a single peak at the expected temperature on the melting curve. The RT reactions were run in triplicate on ninety-six-well reaction plates with the GeneAmp PCR 9700 machine (Applied Biosystems) using TaqMan Reverse Transcription Reagent containing Multiscribe Reverse transcriptase (50 U/μl) (Applied Biosystems). A twofold serial dilution curve (1000–31 ng RNA) of the pooled sample was constructed with six dilutions for the calculation of PCR efficiency. Non-template and non-amplification controls were run in addition to the experimental samples. Total RNA inputs were 250 ng (liver) and 500 ng (intestine) in each RT reaction. Reaction plates with 384 wells were used in which 2 μl of complementary DNA from each RT reaction were mixed with 8 μl of LightCycler 480 SYBR® Green Master Mix (Roche Applied Sciences) with forward and reverse primers (500 nm of each). PCR was achieved with a 5 min activation and denaturation step at 95°C, followed by forty-five cycles of a 15 s denaturing step at 95°C, a 60 s annealing step and a 30 s synthesis step at 72°C. C t values were calculated using the second maximum derivative method in the Light Cycler® 480 software (Roche Applied Sciences). The mean normalised expression of the target genes was determined using a normalisation factor calculated by the geNorm software(Reference Vandesompele, De Preter and Pattyn23) (Biogazelle). Target genes were normalised against an index of the reference genes (ribosomal protein L13A (Rpl13a) and elongation factor 1 (EF1α)). The reference genes were stable with gene expression stability (M) values of 0·41 (liver), 0·68 (mid-intestine, F0) and 0·19 (mid-intestine, F1).
Cyp1A, cytochrome P-450, family 1, subfamily A; CuZn SOD, CuZn superoxide dismutase; ghrelin, ghrelin/obestatin prehormone; MGAM, maltase glucoamylase (α-glucosidase); Slc5a1, sodium/glucose co-transporter (family 5, member 1); PCNA, proliferating cell nuclear antigen; RPL13A, ribosomal protein L13A; EF1α, elongation factor 1α.
Differential leucocyte counts (parental generation)
Within 24 h of sampling, all blood films were stained with the May–Grünwald stain (Merck & Company, Inc.) for 5 min and the Giemsa stain (Merck & Company, Inc.) for 15 min. From each fish sampled, 100 leucocytes were counted and identified either as lymphocytes, granulocytes or monocytes and expressed as a percentage of the total number of leucocytes examined. Each sample was blinded and examined randomly with an Olympus light microscope (BX 51) (Olympus).
Copper zinc superoxide dismutase enzyme activity (parental generation)
Individual liver samples from the parental generation were prepared by adding 500 μl of a cold buffer (20 mm-HEPES, pH 7·2, containing 1 mm-ethylene glycol tetraacetic acid (EGTA), 210 mm-mannitol and 70 mm-sucrose) before being homogenised at 3 × 10 s at 6000 rpm (Precellys 24 homogeniser; Bertin Corp.). The samples were then centrifuged at 10 000 g for 15 min at 4°C before the supernatant was collected and stored at − 80°C for later enzyme analysis. CuZn SOD enzyme activity was assayed according to the assay protocol (SOD assay kit, item no. 706002, Cayman Chemical Company). The absorbance was read at 450 nm using a standard plate reader with a shaker. Using a standard protein assay kit (Pierce® BCA protein assay kit, Thermo Scientific, Pierce Biotechnology), one-third of the supernatant was used for assaying the protein content. The definition of one unit of SOD activity (U) is as follows: the quantity of enzyme required to cause 50 % dismutation of the superoxide radical. The results are expressed as U/min per mg protein.
Fecundity measurements (parental generation)
For the reproductive study, 5-litre breeding tanks equipped with a spawning tray, which consisted of a fine net with an appropriate mesh size for eggs to fall through, close to the bottom of the tank, were used. Males and females from each dietary group were housed separately until the next morning when the light period commenced and they were allowed to breed. The measure of reproductive success was the number of eggs produced by the females per dietary group. Subsequently, after each fecundity experiment, eggs were collected and counted from each group 3 h after the beginning of the light period. Fecundity data are based on groups of females(Reference Knowles2–Reference Then4) mating with three males and are cumulative values that also include the impact of unfertilised eggs.
Analysis of global DNA methylation (offspring generation)
Eggs were carefully rinsed in system water before being incubated with the E3 medium (5 mm-NaCl, 0·17 mm-KCl, 0·33 mm-CaCl2, 0·33 mm-MgSO4 and 0·1 % Methylene Blue) at 29°C, collected at 51 h post-fertilisation and preserved in liquid N2 for later DNA methylation analysis. The total numbers of embryos analysed from each group were 240 (Bt-maize group) and 330 (nBt-maize group). DNA from the embryos was prepared using the method of Skjærven et al. (Reference Skjærven, Hamre and Finn24) as modified by Ramsahoye(Reference Ramsahoye25). Briefly, thirty pooled embryos were thoroughly homogenised in 1 ml of TRIzol (Invitrogen, Life Technologies) using a pestle before homogenising at 3 × 10 s at 6000 rpm (Precellys 24 homogeniser; Bertin Corp.). Total DNA was extracted according to the TRIzol protocol before being further purified and digested into nucleotides(Reference Skjærven, Hamre and Finn24). The samples were stored at − 80°C until further HPLC analyses. Isocratic reverse-phase HPLC was used to analyse the DNA(Reference Skjærven, Hamre and Finn24). Briefly, the mobile phase (20 mm-orthophosphoric acid, pH 2·5) was filtered before use and was run through the HPLC system for approximately 15 min at 0·5 ml/min and 30 min at 1·0 ml/min before each sample series to stabilise the system. The flow of the mobile phase was set to 1 ml/min during the analysis. After each sample series, the HPLC system was washed with 5 % acetonitrile in water for at least 2 h. The samples were run together with nucleotide standards combined in a standard mix. The standard mix consisted of cytosine (dCMP; 2′-deoxycytidine 5′-monophosphate; Sigma D7750), uracil (2,4-dihydroxypyrimidine, Sigma U0750) and methylated cytosine (5mdCMP; 5-methyl deoxycytidine 5′-monophosphate, disodium salt, Reliable Biopharmaceutical product no. 61-1979). Uracil was included in the standard mix as a reference for RNA-free DNA. The percentage of 5-methylcytosine nucleotides was calculated using the following formula(Reference Ramsahoye25):
The molar equivalent of each nucleotide was calculated using the areas under each peak divided by the extinction coefficients for the nucleotides (extinction coefficient for dCMP = 9300 and mdCMP = 8600).
Analysis of the swimming activity of larvae (offspring generation)
At 4 dph, the F1 larvae were placed individually in wells of a ninety-six-well plate containing the E3 medium, and swimming activity was measured using the ZebraLab Quantization software (Viewpoint Life Sciences) equipped with an IR light source, a high-resolution digital IR camera and a hood to exclude external light. Swimming activity was measured for 60 min with alternating light and dark cycles of 10 min. Movement was captured within predefined areas (freezing area, low-movement activity; mid-area, medium-movement activity; burst area, high-movement activity), and output parameters were duration and counts within each area. The sum of total duration was always 60 min. Each time the larvae moved from one area to another, one count was registered, and the counts varied from 100 in slow larvae to 10 000 in active larvae. The total numbers of larvae analysed for each group were 131 (Bt-maize group) and 281 (nBt-maize group).
Histological evaluation of zebrafish intestines (offspring generation)
From the paraffin-embedded intestinal tissues, longitudinal and/or transverse sections (3 μm) were cut and stained with haematoxylin and eosin and mounted on glass microscope slides. Intestinal tissues (proximal intestine and mid-intestine) of all the sections were blinded and evaluated by trained personnel using a light microscope (Carl Zeiss, Inc.), and images were captured using the AxioVision Rel. 4.7 software (Kemet International Limited). Morphology was evaluated according to the following criteria: (1) enterocyte nucleus position; (2) enterocyte vacuolisation; (3) submucosal width and cellularity; (4) lamina propria width and cellularity; (5) intraepithelial leucocyte frequency; (6) enterocyte hyperplasia; (7) goblet cell frequency; (8) presence of mucosal fold fusion. Serial sections were evaluated when necessary. The degree of histological changes was assessed as normal, mild, moderate or severe.
Calculations
Statistical analysis
Statistical analysis was conducted using Statistica™ 7 (StatSoft, Inc.) and GraphPad Prism 5 (GraphPad Software, Inc.). A one-way ANOVA (general lineal model) or unpaired t test was used for data obtained from the F1 or F0 generation, respectively. Data were always evaluated to ensure that the criteria for performing the statistical tests were fulfilled (Bartlett's test for equal variances). In cases when the ANOVA showed significant differences, post hoc tests (Tukey's honestly significant difference test or Fisher's least significant difference test) were used to find which groups differed. Data from the histological evaluations were subjected to a contingency analysis. Data obtained from the pooled fish tanks, performance parameters (F0) after 283 d (Bt-maize: n 11; nBt-maize: n 10), CuZn SOD enzyme analysis (Bt-maize: n 11; nBt-maize: n 10), leucocyte counts (Bt-maize: n 6; nBt-maize: n 8) and reproduction parameters, are reported as means with their 95 % CI. All reported P values are two sided and significance was set at P< 0·05.
Results
Diets, performance parameters and gene transcripts – parental generation
The diets were considered nutritionally equivalent except for the presence of the transgenic Cry1Ab protein and elevated levels of mycotoxin DON in the Bt-maize diet and mycotoxins FB1 and AFLB1 in the nBt-maize diet (Table 1). Of more than 300 pesticides analysed, only trace levels of diphenylamine (0·03–0·05 mg/kg) were detected in the two maize diets. Fish in all tanks were fed identical amounts of feed every day according to body mass, and all feed was consumed immediately, indicating good feed acceptance. Mortality was recorded on a daily basis with no mortality recorded until the end of the trial in which two fish died from each of the dietary groups. A total of 159 mg of feed was given to the fish per tank during the first 45 d of the feeding trial. Performance was not affected by the experimental feeds as assessed by body mass increase, fish length, condition factor (CF) and feed conversion ratio (FCR, Tables 3 and 4). After 45 d, body mass ranged from 169 to 188 mg with no significant differences (P= 0·30) being observed between the two feeding groups, and after 283 d, body mass ranged from 481 to 491 mg (Table 4). The CF was 1·0 for both the feeding groups after 45 d, and after 283 d, the CF were 1·1 (95 % CI 1·0, 1·1) for the nBt-maize diet-fed fish and 1·3 (95 % CI 0·9, 1·7) for the Bt-maize diet-fed fish. FCR, which is the ratio of the amounts of feed consumed to fish weight gain, ranged from 0·8 to 0·9 (45 d), indicating good feed utilisation. Liver oxidative status was assessed after 283 d of feeding by investigating CuZn SOD enzyme activity in the parental zebrafish. The specific enzyme activity ranged from 8·2 (95 % CI 6·1, 10·2) to 8·3 (95 % CI 6·3, 10·3) U/min per mg protein with no differences being observed between the groups (Table 4). After 45 d of feeding, blood samples were collected from the adult fish (F0), and lymphocytes, monocytes and granulocytes were counted (Table 4). The lymphocyte mean population ranged from 81 to 89 %, the monocyte population from 9 to 13 % and the granulocyte population from 3 to 5 %. The mean normalised expression of maltase glucoamylase (MGAM), sodium glucose co-transporter (Slc5a1), CuZn SOD, cytochrome P-450 1A (Cyp1A), caspase 6 and ghrelin in the mid-intestine is reported in Table 3. There were no significant differences between the feeding groups for any of the selected transcripts.
BM, body mass; CF, condition factor; FCR, feed conversion ratio; MGAM, maltase glucoamylase; Slc5a1, sodium glucose co-transporter; CuZn SOD, CuZn superoxide dismutase; Cyp1A, cytochrome P-450 1A; ghrelin, ghrelin prehormone.
* Differences between the treatment groups were tested using an unpaired, two-tailed t test (P< 0·05).
† Initial body weight 13 (sd 6) mg and length 12 (sd 2) mm.
‡ Feed intake per fish was calculated based on the total amount of feed given per tank, which was 159 mg/fish. All feed was weighed before feeding.
BM, body mass; CF, condition factor.
* Only males.
Reproduction parameters
Fish fed the nBt-maize diet had the highest mean fecundity with 203 (95 % CI 117, 290) eggs per female, followed by fish fed the Bt-maize diet, which exhibited 16 % lower mean fecundity (Table 5). The percentage of 5-methylcytosine nucleotides in embryos (51 h post-fertilisation) did not differ between the groups (Table 5). The embryos at this developmental stage had between 7·2 (95 % CI 7·1, 7·3) and 7·4 (95 % CI 6·0, 8·9) % of 5-methylcytosine nucleotides. Swimming activity measurements of the F1 larvae at 4 dpf showed that fish from both the feeding groups spent the same amount of time in the high-activity zone, burst zone (burst duration) (Table 5).
* Given as the mean number of eggs produced by F0 females mating with two to four males (following five matings for the Bt-maize group and seven matings for the nBt-maize group).
† Given as the mean of three F0 females (Bt-maize) or four F0 females (nBt-maize).
‡ Results show time spent in the burst zone for the dietary groups in percentage and are given as the mean of larvae from three F0 females (Bt-maize) and four F0 females (nBt-maize): 131 larvae from three females (Bt-maize) and 281 larvae from four females (nBt-maize).
Performance parameters and gene transcripts – offspring generation
Fish in all tanks were fed the same amounts of feed every day according to satiety (F1), and all feed was consumed immediately, indicating good feed acceptance. While the parental zebrafish were subjected to a restricted feeding regimen (e.g. fed according to body mass), the offspring zebrafish were fed according to a pair-feeding regimen (e.g. according to satiety) and were fed approximately 44 % more than their parents. The difference in feeding regimens was clearly reflected in the performance parameters, resulting in a higher body mass increase and a higher CF compared with those in fish from the parental generation (F0) (Tables 3 and 6). Fish from the parental generation exhibited better feed utilisation than those from the offspring generation, resulting in a higher FCR for the offspring fish (Tables 3 and 6). The Bt-maize diet-fed offspring from the Bt-maize diet-fed parents (Bt–Bt) exhibited a significantly higher body mass increase (P= 0·0003) and specific growth rate (P= 0·0005) than the nBt-maize diet-fed offspring from the nBt-maize diet-fed parents (nBt–nBt) and offspring from the cross-over dietary regimen (Bt–nBt) (Table 6). Feed utilisation was different between the feeding groups with a significantly higher FCR (P= 0·02) in offspring fed the cross-over regimen (Bt–nBt) than in the Bt–Bt offspring. The final fish length was independent of the dietary feeding regimens and was between 25 and 27 mm. The Bt–Bt offspring exhibited a significantly higher level of liver caspase 6 (P= 0·01) and a lower level of liver and mid-intestine CuZn SOD (liver P= 0·02 and mid-intestine P= 0·04) than the nBt–nBt offspring (Table 6). There were no significant differences between the feeding groups for any of the other gene transcripts in the mid-intestine.
BM, body mass; CF, condition factor; FCR, feed conversion ratio, FI, feed intake; SGR, specific growth rate; MGAM, maltase glucoamylase; Slc5a1, sodium glucose co-transporter; CuZn SOD, CuZn superoxide dismutase; Cyp1A, cytochrome P-450 1A; ghrelin, ghrelin prehormone, PCNA, proliferating cell nuclear antigen.
a,bMean values within a row with unlike superscript letters were significantly different (P< 0·05; one-way ANOVA).
* Initial body weight 21 (sd 8) mg and length 11 (sd 2) mm.
Histological evaluation of the intestine (offspring generation)
In general, the intestinal epithelium consists of a single layer of column-shaped enterocytes with basally positioned nuclei and mucus-secreting goblet cells. Enteroendocrine-like cells are mainly scattered at the base of the mucosal folds. The lamina propria and submucosa are very thin with few cells present. The mucosal layer is directly ensheathed by inner circular and outer longitudinal smooth muscle cells of the muscularis layer. According to the morphological characteristics, the intestine can be divided into two regions: proximal intestine and mid-intestine. The proximal intestine displays extensive epithelial folding, while the mid-intestine is distinguished by the presence of large supranuclear vacuoles in the enterocytes. Most proximal intestinal samples displayed normal epithelial morphology. Mild changes were exhibited by five samples. No effects of diets, however, were detected (Table 7; Fig. 2(a) and (b)). Among the five samples from the proximal intestine, two samples (nBt–nBt and Bt–Bt) exhibited mild enterocyte hyperplasia accompanied by increased goblet cell frequency. The presence of intraepithelial leucocytes was slightly increased. The nBt–nBt sample also displayed a mild degree of mucosal fold fusion, and the Bt–Bt sample exhibited widened lamina propria accompanied by connective tissue hyperplasia. The other three proximate intestinal samples (two nBt–nBt samples and one Bt–nBt sample) mainly displayed mild increases in intraepithelial leucocyte frequency with or without widened lamina propria. Taking the enterocyte supranuclear vacuolisation into account, nine of twenty-one mid-intestinal samples exhibited mild morphological alterations. No effects of diets were detected (Table 7; Fig. 2(c) and (d)). Mild inflammatory changes were exhibited by one Bt–Bt mid-intestinal sample, indicated by the increased presence of intraepithelial leucocytes accompanied by widened lamina propria and increased number of goblet cells and decreased supranuclear vacuolisation in enterocytes. The other eight samples with mild changes only exhibited mild-to-moderate decreases in enterocyte supranuclear vacuolisation. No changes were observed in the distal intestine (data not shown).
* Values signify the number of zebrafish per dietary treatment that displayed the various degrees of morphological changes in the proximal intestine and mid-intestine.
† Differences between the treatment groups were tested using a contingency analysis, and P values are given.
‡ Some segments of the intestine were damaged during the processing and explain the different number for the two intestinal segments.
Discussion
To our knowledge, this is the first report on a cross-generational Bt-maize feeding trial in a teleost fish. Based on the parameters investigated, no long-term adverse effects of Bt-maize in either the F0 generation or the F1 generation were observed, indicating that a 19 % inclusion level was either non-toxic or did not result in responses detectable with the analytical methods used or visible with a light microscope. Because zebrafish have a short generation time and are relatively easy to breed, this model was selected to potentially reveal specific target endpoints that could be used to assess the long-term effects of Bt-maize ingredients in aquaculture feeds. The present feed production technique using only low temperatures (40°C) was also more likely to prevent possible heat inactivation of the Cry1Ab protein compared with commercial extruded fish feeds(Reference Sanden, Berntssen and Krogdahl11, 26). Although the exact Cry1Ab protein level in Bt-maize (MON810) is dependent on the growth stage of the plant and the plant tissue, an average content of Cry1Ab of 300 ng/g wet weight of harvested grains has been reported(Reference Nguyen and Jehle27). However, any Cry1Ab present locally in the intestine of zebrafish did not appear to negatively influence growth, intestinal functional gene expression or histomorphology. Nor did any possible absorbed Cry1Ab appear to adversely affect systemic parameters: (1) leucocyte counts indicated predominantly lymphocytes, with an overall mean proportion of 84 %, which is slightly higher than the mean values reported by Murtha et al. (Reference Murtha, Qi and Keller28), but well within the normal range reported for zebrafish lymphocytes, which is between 71 and 92 %(Reference Murtha, Qi and Keller28); (2) levels of gene transcripts involved in DNA repair, detoxification, oxidative stress and apoptosis in the liver were apparently not adversely affected; (3) reproductive parameters were not affected.
Interestingly, offspring zebrafish fed the Bt-maize diet exhibited enhanced growth performance than those fed the nBt-maize diet, as indicated by higher specific growth rate and body mass increase. Although no significant differences were observed in the parental generation (F0), the same trends were observed. The difference between the generations may be explained by the use of ad libitum feeding regimen in the offspring fish (F1) as opposed to a restricted feeding regimen for the F0 generation. Despite not being significant in the parental generation (F0), the numerical difference was in the same direction for the F0 generation. The Bt–Bt offspring had significantly decreased expression levels of CuZn SOD in both the liver and mid-intestine, which may indicate reduced oxidative stress in these tissues, than the nBt–nBt offspring. Offspring fish fed the Bt-maize diet also exhibited higher gene transcript levels of hepatic caspase 6, which may indicate that pathways in the cell cycle were affected by dietary factors. However, for the other gene biomarkers, no significant differences were observed. Nor were diet-related histomorphological changes in the intestine observed. Another study, which focused on the long-term effects in Bt-maize-fed pigs, found no local or systemic allergic or inflammation-type immune responses(Reference Walsh, Buzoianu and Rea29). Enhanced growth performance in zebrafish fed Bt-maize than in those fed nBt-maize has also been observed in a previous trial(Reference Sissener, Johannessen and Hevroy7) where ad libitum feeding was used.
Increased growth with Bt-maize feeding than with nBt-maize one has also been reported for other animal species and has been hypothesised to be due to reduced DON content in Bt-maize(Reference Flachowsky, Chesson and Aulrich30). Clearly, this was not supported in the present study since DON levels in the Bt-maize diet were higher than those in the nBt-maize diet (Table 1). Furthermore, lack of DON effects on growth performance has recently been reported in another zebrafish trial, in which concentrations of DON much higher than those used in the present study were used(Reference Sanden, Jorgensen and Hemre14). In the previous zebrafish study(Reference Sissener, Johannessen and Hevroy7), reduced mycotoxin levels in Bt-maize were also speculated to be the cause of the enhanced growth. However, retrospective analysis of the maize used in that study revealed that Bt-maize in fact had a higher DON content than nBt-maize(Reference Sissener, Lall and Sagstad13). Consequently, those results are similar to the ones presented here, making it less likely that these are random findings, although the cause is not clear.
On the other hand, the nBt-maize diet contained low, but detectable levels of AFLB1 and FB1 than the Bt-maize diet. Thus, it cannot be ruled out that these mycotoxins may have contributed to the reduced growth and other responses in the nBt-maize diet-fed fish. For fumonisins, a non-observable effect level for feed was set to 3 mg/kg for rainbow trout(Reference Carlson, Williams and Spitsbergen31), and for AFLB1, it has been reported that 0·4 μg/kg feed can cause haematomas when fed to rainbow trout for 15 months(Reference Lee, Wales and Ayres32). In the nBt-maize diet used in the present study, the level of AFLB1 was 0·4 μg/kg and the level of FB1 was 23 μg/kg. Although the individual levels of AFLB1 and FBI were low in our diets, synergism has been reported for these two mycotoxins with decreased body weight gain as the most frequently reported effect(Reference Pedrosa and Borutova33). Fumonisins are inhibitors of ceramide synthase, a key enzyme in lipid metabolism, and as a consequence the levels of free sphingoid bases may be elevated. Free sphingoid bases have been found to be toxic to most cells by affecting cell proliferation and inducing apoptosis or necrotic cell death(Reference Yoo, Norred and Showker34). Aflatoxins, on the other hand, may act as carcinogens by forming DNA adducts and could affect apoptosis and cell proliferation by causing mutations in these genes(Reference Santacroce, Conversano and Casalino35). In the present study, a decreased liver gene transcript level of caspase 6 (execution phase of apoptosis) was observed concomitant with an increased liver and mid-intestinal gene transcript level of CuZn SOD in the nBt–nBt offspring. Higher liver gene transcript levels of Cyp1A in these fish were also observed, but they were not significant due to large variations between the tanks within the same dietary group. Thus, the decreased growth in the nBt-maize groups may indicate changed energy metabolism due to, for example, energy-demanding processes such as cellular detoxification, increased cellular proliferation/apoptosis and/or oxidative stress. Further control groups could have made it easier to understand and explain the unexpected differences observed between the two groups, but such groups were not possible to obtain in the present study. Overall, however, the growth performance in the present study was comparable to that reported in other studies using non-commercial diet formulations(Reference Sissener, Johannessen and Hevroy7, Reference Sanden, Jorgensen and Hemre14, 36). Compared with the growth performance of zebrafish fed commercial diets and live feed, the growth observed in the present study was lower in both the feeding groups(Reference Gomez-Requeni, Conceicao and Jordal37).
Other targets in the present study were the reproductive performance of the parental generation (fecundity), offspring larva swimming behaviour and DNA methylation in embryos. Reproductive performance has also been investigated in mice fed Bt-maize with a focus on testicular development. Ingestion of Bt-maize by mothers during pregnancy and later by the young developing male mice had no negative effects on fetal, postnatal, pubertal or adult testicular development or body growth(Reference Brake, Thaler and Evenson38). The overall mean number of eggs produced by the zebrafish was 189, which corresponds to what has been reported in the literature. The present study found no differences between the feeding groups. In the present study, DNA isolated from embryos obtained from the exposed parental generation was analysed using HPLC to determine the relative amount of cytosine and 5-methylcytosine nucleotides. Methylation of cytosine is an important mechanism that affects the transcription of genes. Changes in global DNA methylation may also result from impaired absorption of nutrients due to intestinal damages(Reference Hunder, Schümann and Strugala39). However, we found no effect on global DNA methylation in the F1 progeny, which ranged from 7·2 to 7·4 % across both the groups. The level of DNA methylation in the present study was slightly lower than what has been reported previously for adult zebrafish liver, which was above 8 %(Reference Mirbahai, Williams and Zhan40). In the present study, F1 larva swimming activity measurements were evaluated by investigating offspring larva activity. Movement was captured within the predefined areas, and output parameter was duration within the high-activity zone. It has been suggested that it is a disadvantage for the fish to show increased activity at this yolk-sac stage as it may negatively affect further growth and development(41). We found no effects on larva swimming activity in the present study.
Conclusion
We found no adverse performance or reproductive effects in zebrafish fed the Bt-maize diet for two generations, and Bt-maize seems to be as safe and nutritious as its nBt-maize control. It is emphasised that parameters related to potential allergenic reactions from the Cry1Ab protein were not investigated. The differences observed in contamination with mycotoxins (FB1 and AFLB1) between Bt-maize- and nBt-maize-containing diets may explain the effects observed on gene transcript biomarkers in pathways of the cell oxidative system and the cell cycle in fish fed the nBt-maize diet for two generations.
Acknowledgements
The present study was supported by the Norwegian Ministry of Fisheries and Coastal Affairs and also partially supported by a European Union Seventh Framework Programme grant (GMSAFOOD, grant no. 211820). The authors thank Øyvind Reinshol at their zebrafish research laboratory for skilled animal care and Eva Mykkeltveit, Hui-Shan Tung and Synne Wintertun for their excellent technical assistance. They also thank Kaja Skjærven for valuable discussions and input on fertilised zebrafish egg ontogeny and the DNA methylation method and Ståle Ellingsen for helping with the zebrafish swimming activity measurements. M. S., N. H. S. and G.-I. H. designed the study. M. S. designed and prepared the feeds. M. S., N. H. S., G.-I. H. and S. J. participated in the sampling. M. S. and S. J. conducted the laboratory analysis. J. G. conducted the histomorphological evaluations. M. S. and R. O. conducted the DNA methylation analysis. M. S. wrote the manuscript. All authors read and approved the final manuscript. The authors declare no conflicts of interest.