Microinjection procedure

Fertilised zebrafish eggs were obtained from natural spawning of wild-type breeding fish (Centre of Marine Sciences). Embryos were injected into the yolk with 4·6 nl of either a saline solution (Danieau) or 2 m-glucose solution, at the late embryo stage of 1 dpf (during the pharyngula period, according to the method described by Kimmel et al. ⁽ Reference Kimmel, Ballard and Kimmel ^{22 )}). Solutions were prepared according to the procedures described by Rocha et al. ⁽ Reference Rocha, Dias and Engrola ^{17 )}. Microinjection was performed using a 0·5 mm-diameter glass capillary inserted on a nanolitre injector (World Precision Instruments) following the same procedures as described by Rocha et al. ⁽ Reference Rocha, Dias and Engrola ^{17 )}.

Fish rearing and experimental feeds

The present experiment was carried out in compliance with the Guidelines of the European Union Council (2010/63/EU) legislation for the use of vertebrate animals^{( 23 )}. After glucose and saline injections (described above), embryos and larvae were raised in triplicate tanks (n 200) at an initial density of 100 larvae/l, under standardised conditions (28°C) as described previously by Westerfield⁽ Reference Westerfield ^{24 )}. An additional group of non-injected embryos was reared simultaneously to monitor egg quality and embryonic development. From 5 dpf, larvae were fed Artemia nauplii, which were gradually replaced by an inert diet from 10 to 15 dpf. After day 15, larvae were fed exclusively on a low-carbohydrate high-protein (LC) diet used as the control (Fig. 1). From 25 to 35 dpf, all fish from both injection treatments were subjected to a dietary challenge with a high-carbohydrate low-protein (HC) diet (Fig. 1). Throughout the trial, larvae and juvenile zebrafish were fed by hand (four meals/d) until visual satiation. Both diets were well accepted by the fish. Fish mortality was daily monitored, and survival rate was determined at the end of the trial.

Fig. 1 Experimental set-up for zebrafish rearing and feeding regimen up to 35 d post-fertilisation (dpf). Embryos were injected into the yolk at 1 dpf either with a saline or 2 m-glucose solution. At the beginning of exogenous feeding, larvae were fed with Artemia nauplii, which were gradually replaced by a low-carbohydrate high-protein (LC) control diet. Juveniles were subjected to a 10 d dietary challenge, being fed exclusively on a high-carbohydrate low-protein (HC) diet. Sampling points for the metabolic trial and gene expression were marked. Age is expressed as dpf at 28°C.

Formulation of the experimental diets was based on the use of purified ingredients in order to guarantee a high control of nutritional changes among the diets (Table 1). The LC control diet had a high incorporation level of concentrated protein sources (casein, soya isolate, wheat gluten and fish gelatin), guaranteeing a high level of crude protein (70 %) and a low level of carbohydrates (6 %). In the HC (or challenge) diet, the crude protein level was drastically reduced (25 %), whereas carbohydrate level (51 %) was increased through the incorporation of maize dextrin, a highly digestible carbohydrate. Both diets were isolipidic (12 %) and dully supplemented with selected crystalline indispensable amino acids and monocalcium phosphate to avoid essential amino acid or phosphorus imbalance. The experimental diets were manufactured by SPAROS Lda. Powder ingredients were grinded (below 100 μm) in a micropulveriser hammer mill (Hosokawa Micron). Powder ingredients and oil sources were then mixed accordingly to the target formulation in a mixer (Sammic BM5E), and the mixture was humidified with 25 % water. The diets were manufactured by temperature-controlled extrusion (pellet size 2·0 mm) by means of a low-shear extruder (Italplast P55). Upon extrusion, all feed batches were dried in a convection oven (OP 750-UF; LTE Scientifics) for 3 h at 40°C. Dry feed pellets were then grinded in a coffee mill and sieved manually to retrieve the desired particle size (100–200 and 200–400 μm). The diets were analysed for proximate composition according to the following procedures: DM after drying at 105°C for 24 h; ash content by incineration in a muffle furnace at 500°C for 12 h; crude protein (N × 6·25) by a flash combustion technique followed by a gas chromatographic separation and thermal conductivity detection (LECO FP428); fat by dichloromethane extraction (Soxhlet); gross energy in an adiabatic bomb calorimeter (IKA C2000); total phosphorus according to the ISO/DIS 6491 method using the vanado-molybdate reagent.

Table 1 Formulation and composition of the low-carbohydrate high-protein (LC) control and the high-carbohydrate low-protein (HC) challenge diets

* Pharma Grade bloom 240: 92 % CP, LAPI Gelatine SPA.

† Edible acid casein 90 mesh: 85 % CP, EPI Ingredients.

‡ SEAH Soy Instant: 87 CP%, Seah International.

§ VITEN: 86 % CP, 1·3 %, Roquette.

∥ TACKIDEX C070: Roquette.

¶ Marine oil omega-3: Henry Lamotte Oils GmbH.

** PREMIX Lda. Vitamins (mg/kg diet): dl-α-tocopherol acetate, 100 mg; sodium menadione bisulphate, 25 mg; retinyl acetate, 6·9 mg; dl-cholecalciferol, 0·05 mg; thiamin, 30 mg; riboflavin, 30 mg; pyridoxine, 20 mg; cyanocobalamin, 0·1 mg; nicotinic acid, 200 mg; folic acid, 15 mg; ascorbic acid, 1000 mg; inositol, 500 mg; biotin, 3 mg; calcium pantothenate, 100 mg; choline chloride, 1000 mg; betaine, 500 mg. Minerals (g or mg/kg diet): cobalt carbonate, 0·65 mg; copper sulphate, 9 mg; ferric sulphate, 6 mg; potassium iodide, 0·5 mg; manganese oxide, 9·6 mg; sodium selenite, 0·01 mg; zinc sulphate,7·5 mg; NaCl, 400 mg; calcium carbonate, 1·86 g; excipient wheat middlings.

†† Monocalcium phosphate: 22 % P, 16 % Ca, Fosfitalia.

‡‡ Sigma-Aldrich Quimica SA.

§§ Carbohydrate content calculated as: 100–(moisture+protein+fat+ash).

Biological and analytical sampling

Immediately after injection, samples (n 30) of glucose- and saline-injected eggs were collected for the analysis of glucose levels by fluorescent spectroscopy using a commercial kit (Amplit Glucose Quantitation Kit; AAT Bioquest). Fluorescence readings were performed in triplicate using a Synergy™ 4 Multi-Mode Microplate Reader controlled by Gen5™ software (BioTek Instruments). At the end of the experiment (35 dpf), juveniles (n 20 per treatment) were individually sampled for growth determination based on dry weight and total length parameters. Total length was determined using the AxioVision 4.8.2 (Carl Zeiss Limited) program for image analysis, and dry weight measurements were obtained from freeze-dried samples using a precision scale. For gene expression analysis, samples of whole-body larvae (n 20) from each replicate of glucose- and saline-injected treatments were collected during the endogenous feeding period (4 dpf). At the end of the trial, liver and muscle from individual fish (n 6 per treatment) were sampled 6 h after feeding for the same purpose. All samples were randomly collected, snap-frozen in liquid N₂ and kept at (80°C until analysis.

Metabolic trial

Tube-feeding method

At 1 d before the final sampling (34 dpf), juveniles from each treatment (n 10) were randomly harvested from the tanks and transferred to the flux laboratory for overnight acclimatisation at room temperature (28°C). Fish were deprived from feed for 16 h before the metabolic trail. The in vivo method of controlled tube-feeding, as described by Rust et al. ⁽ Reference Rust, Hardy and Stickney ^{25 )} and later modified by Rønnestad et al. ⁽ Reference Rønnestad, Rojas-Garcıa and Tonheim ^{26 )}, for marine fish was adapted to supply nutrients to freshwater species. This approach was used to assess the effects of both nutritional conditioning (early glucose injection) and increase in dietary carbohydrates on the metabolic handling of glucose by zebrafish juveniles. Following a 16 h fasting period, zebrafish juveniles were allowed to feed on the HC diet for a period of 40 min. This feeding period was suitable for the uptake of a full meal, as confirmed by observation of the gastrointestinal tract, and within the beginning of the zebrafish gastrointestinal transit⁽ Reference Field, Kelley and Martell ^{27 )}. Following this single meal, fish were anaesthetised with 33 μm-tricaine methanesulfonate (Sigma-Aldrich). Subsequently, the radioactive label d-[¹⁴C(U)]glucose (9·25 MBq; American Radiolabeled Chemicals, Inc.) was added to Ringer salt solution and tube-fed to all fish using a 0·19 mm-diameter plastic capillary (Sigma-Aldrich) inserted on a nanolitre injector (World Precision Instruments). Thereafter, three consecutive injections of 4·6 nl were administered into the fish gut. This injection volume (13·8 nl) was in the range of that previously used for marine species in late larval stages (>25 d after hatching): Senegalese sole⁽ Reference Aragão, Conceição and Martins ^{28 ,} Reference Morais, Koven and Rønnestad ^{29 )}; gilthead seabream⁽ Reference Pinto, Rodrigues and Dinis ^{30 )}; white seabream⁽ Reference Saavedra, Conceição and Helland ^{31 )}. After capillary withdrawal, fish were gently rinsed for spillage through two successive wells filled with clean freshwater and transferred into sealed incubation chambers containing 6·5 ml of freshwater. The incubation water was considered to contain all labelled ¹⁴C resulting from fish evacuation (evacuated fraction). In addition, an airflow connection was provided between each incubation chamber and a KOH trap (5 ml, 0·5 m), in order to collect all ¹⁴CO₂ released by the fish through glucose metabolism (catabolised fraction). After an incubation period of 24 h, juveniles from each injection treatment were sampled individually for muscle and viscera, in order to determine the amount of ¹⁴C retained in tissues (retained fraction). Tissue samples were immediately solubilised with Solvable (500 μl; PerkinElmer) and kept at 50°C for 24 h. Following larval sampling, the incubation chambers were resealed and 1 ml HCl (0·1 m) was added in a series of gradual steps, resulting in a progressive decrease of pH that causes the rapid diffusion of any remaining ¹⁴CO₂ from the water into the metabolic trap (catabolised fraction)⁽ Reference Rønnestad, Rojas-Garcıa and Tonheim ^{26 )}. For radioactive counting, dpm were determined in all samples by adding the Ultima Gold XR scintillation cocktail (PerkinElmer) and counting in a TriCarb 2910TR Low Activity Liquid Scintillation analyser (PerkinElmer). Metabolic budgets were calculated after subtracting blanks of each fraction (evacuated, catabolised and retained). Results for each fraction are expressed as a percentage of total label tube-fed, i.e. the sum of dpm in all the compartments of the metabolic chamber and fish.

Gene expression analysis

Real-time PCR

Analyses of mRNA levels were performed at two distinctive periods and sample types: at 4 dpf in whole-body larvae, for assessing the short-term effect of early glucose stimulus (injection), and at 35 dpf in the visceral and muscle tissues of juveniles, for assessing the effects of both early glucose stimulus and dietary challenge. Juvenile fish were sampled 6 h after the last meal, based on previous data identifying this period as relevant for examining the postprandial response of genes in zebrafish⁽ Reference Amaral and Johnston ^{32 ,} Reference Seiliez, Medale and Aguirre ^{33 )}. Total RNA was extracted from all samples using 1 ml TRIzol^® reagent (Invitrogen). From the resulting total RNA, 1 μg was reverse transcribed into complementary DNA using the SuperScript III RNase H Reverse Transcriptase Kit (Invitrogen) with random primers (Promega). Molecular analysis was focused on the expression of target genes related to glycolysis (GK, glucokinase; HK1, hexokinase 1; 6PFK, phosphofructokinase-6; PK-L, PK-M, pyruvate kinase, both liver and muscle isoforms), gluconeogenesis (PEPCK, phosphoenolpyruvate carboxykinase, both cytosolic and mitochondrial isoforms; FBP, fructose-1,6-bisphosphatase; G6Pase, glucose-6-phosphatase), lipogenesis (FAS, fatty acid synthase; G6PDH, glucose-6-phosphate dehydrogenase; MEc, cytosolic malic enzyme) and glycogen metabolism (GS, glycogen synthase; GP, glycogen phosphorylase). These primers were considered as good molecular markers for nutritional studies in zebrafish⁽ Reference Rocha, Dias and Engrola ^{17 ,} Reference Seiliez, Medale and Aguirre ^{33 )}. Gene expression levels were determined by quantitative real-time RT-PCR performed by means of the iCycler iQ (Bio-Rad). Analyses were performed on 5 μl of diluted complementary DNA using the iQ SYBR^® Green supermix in a total PCR volume of 15 μl containing, 200 nm of each primer. Thermal cycling was initiated with the incubation at 95°C for 90 s for Taq DNA polymerase activation, then thirty-five steps of PCR were performed, each one consisting of heating at 95°C for 20 s for denaturing and at 55°C or 62°C for 30 s for annealing and extension, depending on the primers. After the final cycle of the PCR, melting curves were systematically monitored (55°C temperature gradient at 0·5°C/s from 55 to 94°C). Each quantitative PCR run included duplicates of samples (reverse transcription) and negative controls (samples without RT or mRNA or complementary DNA). Target gene expression analysis of whole-body larvae and visceral tissue from juveniles was performed using elongation factor-1 (EF1α) as the reference gene, while 18S rRNA was used as the reference gene for muscle samples, once EF1α was not being stably expressed in this tissue. Both EF1α and 18S were employed as non-regulated reference genes and their gene expression values did not significantly change over the respective time frame or tissue type⁽ Reference McCurley and Callard ^{34 )} (data not shown). Relative quantification of gene expression was performed using the mathematical model described by Pfaffl⁽ Reference Pfaffl ^{35 )}.

Statistical analysis

Data are presented as means with their standard errors of the mean. Criteria expressed as a percentage were arcsine transformed previously to the statistical analysis. The effects of glucose injection on the several analysed parameters in larvae and juvenile fish were tested using SPSS^® statistics software 16.0 for Windows by means of an unpaired two-tailed Student's t test. Differences were considered significant at P< 0·05. For relative quantification of gene expression in juvenile fish, the control group was set as the saline-injected HC diet-fed group.