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Characterisation and expression of secretory phospholipase A2 group IB during ontogeny of Atlantic cod (Gadus morhua)

Published online by Cambridge University Press:  14 September 2010

Øystein Sæle*
Affiliation:
National Institute of Nutrition and Seafood Research, PO Box 2029, Nordnes, 5817Bergen, Norway
Andreas Nordgreen
Affiliation:
National Institute of Nutrition and Seafood Research, PO Box 2029, Nordnes, 5817Bergen, Norway
Pål A. Olsvik
Affiliation:
National Institute of Nutrition and Seafood Research, PO Box 2029, Nordnes, 5817Bergen, Norway
Kristin Hamre
Affiliation:
National Institute of Nutrition and Seafood Research, PO Box 2029, Nordnes, 5817Bergen, Norway
*
*Corresponding author: Ø. Sæle, fax +47 55 90 52 99, email [email protected]
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Abstract

The pancreatic enzyme secretory phospholipase A2 group IB (sPLA2 IB) hydrolyses phospholipids at the sn-2 position, resulting in a NEFA and a lyso-phospholipid, which are then absorbed by the enterocytes. The sPLA2 IB is a member of a family of nineteen enzymes sharing the same catalytic ability, of which nine are cytosolic and ten are secretory. Presently, there are no pharmacological tools to separate between the different secretory enzymes when measuring the enzymatic activity. Thus, it is important to support activity data with more precise techniques when isolation of intestinal content is not possible for analysis, as in the case of small teleost larvae, where the whole animal is sometimes analysed. In the present study, we characterise the sPLA2 IB gene in Atlantic cod (Gadus morhua) and describe its ontogeny at the genetic and protein level and compare this to the total sPLA2 activity level. A positive correlation was found between the expression of sPLA2 IB mRNA and protein. Both remained stable and low during the larval stage followed by an increase from day 62 posthatch, coinciding with the development of the pyloric ceaca. Meanwhile, total sPLA2 enzyme activity in cod was stable and relatively high during the early stages when larvae were fed live prey, followed by a decrease in activity when the fish were weaned to a formulated diet. Thus, the expression of sPLA2 IB mRNA and protein did not correlate with total sPLA2 activity.

Type
Full Papers
Copyright
Copyright © The Authors 2010

Phospholipids (PL) are an essential nutrient for fish larvae (see review by Coutteau et al. (Reference Coutteau, Geurden and Camara1)), and it has been demonstrated in fish larvae that increasing dietary PL levels can improve growth rates, increase survival(Reference Radunzneto, Corraze and Charlon2Reference Cahu, Infante and Barbosa4), reduce deformation(Reference Cahu, Infante and Barbosa4) and improve stress tolerance(Reference Kanazawa5). Generally, the dietary requirement of PL is high in fish larvae at the start of feeding and decreases as the fish approach the juvenile stage(Reference Geurden, Coutteau, Sorgeloos, Lavens and Jaspers3, Reference Kanazawa5, Reference Cahu, Gisbert and Villeneuve6). Although it is well known that the digestive system in altricial fish is still developing during the larval stage, it is still uncertain why there is such a high PL requirement during this period. Furthermore, it has been demonstrated that the digestive tract of sea bass (Dicentrarchus labrax) larvae matured faster and the larvae had increased growth, survival and decreased malformations when fed compound diets containing high levels of dietary PL from first feeding(Reference Cahu, Infante and Takeuchi7). The same study also suggests that sea bass utilise dietary PL more efficiently than neutral lipids.

Digestion of PL is mainly catalysed by pancreatic phospholipase A2 (phosphatide 2-acyl hydrolase, EC 3.1.1.4; PLA2). The PLA2 hydrolyses the fatty acid ester bond at the sn-2 position of PL and produces a NEFA and a lysophospholipid(Reference Izquierdo, Socorro and Arantzamendi8). Altogether, nineteen enzymes with PLA2 activity have been described in mammals. Ten of these are of the secretory type and nine are cytosolic. One of the secretory PLA2 (sPLA2) is produced in the pancreas for the purpose of PL digestion: the sPLA2 IB(Reference Murakami and Kudo9). All the sPLA2 are Ca2+ dependent and are recognised by a conserved Ca2+-binding loop as well as a conserved catabolic site. The distinctive feature separating the pancreatic form sPLA2 IB involved in PL digestion from the other sPLA2 is a domain called the pancreatic loop.

Unfortunately, there are no methods available today to distinguish between the enzymatic activities of the different PLA2 ; at best, it is possible to discriminate between the cytosolic and secretory forms(Reference Hendrickson, Hendrickson and Dybvig10, Reference Reynolds, Hughes and Dennis11). This presents a challenge when analysing small marine larvae where dissection of the digestive tract may be challenging, and therefore whole fish must be analysed. The analysis of PLA2 activity in whole fish larvae will provide information of PL hydrolysis in all tissues involving a multitude of sPLA2 enzymes, which will obscure information of the digestive capability of specific phospholipases. It is therefore vital to accompany enzymatic activity analysis with more specific protein and mRNA quantification methods describing the enzyme in question.

Two low-molecular-weight sPLA2 group IB have been characterised in the hepatopancreas of red sea bream (Pagrus major)(Reference Iijima, Fujikawa and Tateishi12), and there is also a description of a PLA2 in sea bass(Reference Cahu, Infante and Barbosa4). Little information on the ontogeny of PLA2 activity in marine fish larvae is available, but Uematsu et al. (Reference Uematsu, Kitano and Morita13) did not find PLA2 in acinar cells of the hepatopancreas in red sea bream before 13 d post hatch (dph). To shed light on the dynamics of sPLA2 IB ontogeny in fish larvae, we have analysed the enzyme at the mRNA and protein level and compared this to total sPLA2 activity. Due to multiplicity of enzymes in the PLA2 family, we have emphasised the description of the distinctive parts of the pancreatic form of PLA2. Furthermore, we discuss what different analytical tools may reveal about the production and activity of this one specific enzyme out of the multitude of other similar enzymes.

Material and methods

Biological parameters

Atlantic cod (Gadus morhua) larvae were sampled from three production tanks at the commercial hatchery Cod Culture Norway, in Rong, Norway, according to their fish holding routines, which are in accordance with the Animal Welfare Act of 12 December 1974, nr 73, §§22 and 30, amended 17 November 1998. Eggs were collected from natural spawning brood stock and incubated for 15 d at 7°C. Hatched embryos were transferred to three start feeding tanks (diameter: 3 m, depth: 1 m) and fed rotifers (Brachionus plicatilis) from 3 dph. Formulated diet (Gemma Micro, Skretting, Norway) was introduced to cod larvae at 18 dph and co-fed with rotifers until 30 dph. From 31 dph and onwards, larvae were fed solely on formulated diet. Fertilised eggs used for the production of larvae used in this work came from a brood stock tank containing fifty-five females and thirty-nine males. The batch of eggs may therefore come from multiple parents. The temperature in the three sampling tanks was 7·1 ± 1°C at 3 dph and was raised incrementally to 11°C by 17 dph. The temperature was kept constant at 11·2 ± 0·5°C for the rest of the sampling period. Oxygen was measured and delivered continuously to larval tanks via an automated system with oxygen saturation ranging from 84 to 97 % within tanks during the sampling period.

Biological sampling

Pooled samples of whole larvae and/or larvae gastrointestinal tract (GI-tract) were taken from the three tanks at every sampling point (Fig. 1) from 3 to 62 dph. At 74 dph, the three fish tanks were graded and approximately 35 % of the smallest fish were removed. This was routinely done at the commercial facility where we sampled the larvae. The retained fish were sorted into a medium- and large-sized group. At 83 and 97 dph, fish were sampled from both the medium- and large-size group. Until 56 dph, the fish were collected using a 60 cm long glass pipette. From 63 dph, the fish were collected using a fish net. Fish were collected from approximately 40 cm below the surface and from the areas in the tank with the highest density of fish. The larvae were filtered using a plankton net screen which was patted dry from underneath with a paper towel to remove excess water from the larvae. All the larvae were killed by inserting a needle through the brain before dissection. The whole larvae were then collected in 1·5 ml Eppendorf tubes. The GI-tract was sampled by cutting off the head in a backward angle following the gills. This incision cut the oesophagus without spilling the stomach content. The intestinal tract was detached from the body cavity by an incision anterior to the anus opening, and then the GI-tract was carefully pulled out. The liver was carefully removed, but all other intestinal organs were included with the GI-tract samples. Whole larvae were sampled from 3 to 62 dph and the digestive tract was sampled from 34 to 98 dph (Fig. 1).

Fig. 1 Trial and sampling scheme. The arrow gives the type of diet during the sampling period, numbered circles indicate the number of pooled individuals in each sampling and the age of larvae at sampling is given in days post hatch (dph). GI, gastrointestinal tract.

For RNA extraction, whole larvae or dissected GI-tract were pooled and homogenised with a pestle mortar in Eppendorf tubes containing 1 ml Trizol (Invitrogen Life Technologies, Carlsbad, CA, USA). The samples were then put on dry ice for approximately 3–5 h before storing at − 80°C until RNA extraction. For enzyme activity and Western blot, larvae and GI-tract samples were flash-frozen in liquid N2 without any treatment. At every sampling point, standard length (SL) (minimum ten fish/tank) was measured. Fish weight was measured from 56 dph (fifteen fish/tank). The fish were dried with paper and weighed individually. All the fish sampled for measuring length (SL) and weight were anaesthetised and killed with an overdose of metacaine (MS-222™; Norsk medisinaldepot AS, Bergen, Norway) dissolved in seawater. Dry weight was calculated according to Finn et al. (Reference Finn, Ronnestad and van der Meeren14) based on SL. A size- and temperature-based growth model was used to evaluate the growth performance according to Folkvord(Reference Folkvord15).

RNA extraction and quantitative PCR

The homogenised and stored in Trizol samples were thawed and thoroughly homogenised a second time, using a Precell 24 (Bertin Technologies, Montigny le Bretonneux, France). Total RNA was extracted from whole fish and GI-tract with Trizol reagent (Invitrogen Life Technologies), according to the manufacturer's instructions. The RNA-isolated samples were diluted in RNase-free double-distilled H2O to 200 mg/μl and treated with DNA-free TM kit (Ambion, Austin, TX, USA) according to the manufacturer's descriptions. The quality of the RNA was assessed with the NanoDrop® ND-1000 UV–Vis Spectrophotometer (NanoDrop Technologies, Wilmington, DE, USA). Optical density 260 nm/optical density 280 nm ratios for all total RNA samples ranged between 1·87 and 2·06.

Integrity of the RNA was controlled in twelve randomly chosen samples out of the thirty-six using the Agilent 2100 Bioanalyzer (Agilent Technologies) and the RNA 6000 Nano LabChip® kit (Agilent Technologies, Palo Alto, CA, USA). RNA integrity numbers(Reference Mueller, Hahnenberger and Dittmann16, Reference Imbeaud, Graudens and Boulanger17) were between 8·9 and 10.

RT-PCR were run in duplicates on a ninety-six-well plate. For efficiency calculations, a twofold serial dilution of total RNA, mixed from all samples, ranging from 1000 to 31 ng/μl, was run in triplicates. All reactions were synthesised with a 500 ng total RNA input. Each plate included a no template control and RT-control (a reaction without RT enzyme). Plates were run on a GeneAmp PCR 9700 (Applied Biosystems, Foster City, CA, USA) using TaqMan Reverse Transcription Reagent containing Multiscribe RT (50 U/μl; 833·5 nkat/μl) (Applied Biosystems).

Reverse transcription was performed at 48°C for 60 min by using oligo dT primers (2·5 μm) for all the genes in 30 μl total volume. The final concentrations of the other chemicals in each RT reaction were MgCl2 (5·5 mm), dNTP (500 mm of each), 10 ×  TaqMan RT buffer (1 × ), RNase inhibitor (0·4 U/μl) and Multiscribe RT (1·67 U/μl).

From each RT reaction, 2 μl of complementaryDNA and then 18 μl consisting of 7·6 μl double-distilled H2O, 10 μl TaqMan® Universal PCR Master Mix (Applied Biosystems), 0·2 μl of each primer (50 μm forward: GTCACGGTCTTGGTGCTCTTG and reverse: GCCAAACTCATGACCATTGCT) were pipetted in duplicate to 384-well plates. Pipetting was performed automatically by a robot (Biomek 3000; Beckman Coulter, Fullerton, CA, USA). Real-time PCR was run on the LightCycler® 480 Real-Time PCR System (Roche Applied Sciences, Basel, Switzerland), with a 5 min activation and denaturing step at 95°C, followed by forty cycles of a 15 s denaturing step at 95°C, a 60 s annealing step and a 30 s synthesis step at 72°C. The annealing temperature was 60°C for all primer pairs.

For the mean normalised expression calculations of the target genes, the geNorm VBA applet for Microsoft Excel 97 was used to calculate a normalisation factor based on three reference genes(Reference Vandesompele, De Preter and Pattyn18). Ubiquitin, RPL 4 and RPL 37 were the selected reference genes based on Olsvik et al. (Reference Olsvik, Softeland and Lie19) and Sæle et al. (Reference Saele, Nordgreen and Hamre20), and the normalising factor calculated from these genes was used to calculate the mean normalised expression for each of the target genes.

Homogenisation

Whole larvae and dissected GI-tracts were homogenised in 4 ×  sample wet weight PBS with an Ultra – Turax® 20 000 (Upm, Janke u. Kunkel KG, Germany) followed by a second homogenisation in a ball mill (Retsch® MM301; Retsch GmbH, Haan, Germany), for 2 × 2 min (thirty shakes/s). Homogenates were centrifuged at 10 000 g for 15 min at 4°C and the supernatants were measured for total protein with the BCA Protein Assay Kit (Thermo Fisher Scientific, Inc., Rockford, IL, USA), according to the manufacturer's instructions. The supernatant was used for analysis of enzyme activity and for Western blot analysis.

Enzyme activity

A sPLA2 assay kit (product no. 765001; Cayman Chemical Company, Ann Arbor, MI, USA) was used for enzyme activity calculations. The assay uses the 1,2-dithio analogue of diheptanoyl phosphatidylcholine which serves as a substrate for most PLA2 (for example, bee and cobra venoms, pancreatic fluid, etc.) with the exception of cytosolic PLA2 (Reference Hendrickson, Hendrickson and Dybvig10, Reference Reynolds, Hughes and Dennis11). Upon hydrolysis of the thio-ester bond at the sn-2 position by PLA2, free thiols are detected using 5,5-dithio-bis-(2-nitrobenzoic acid). Plates were read every 15 s for 30 min at 414 nm with a microreader (Labsystems iEMS Reader MF, Helsinki, Finland). Enzymatic activity was calculated accordingly:

ΔA 414/ min  is the change in absorbance/min, 10·66 per mm is the extinction coefficient for 5,5-dithio-bis-(2-nitrobenzoic acid) under the assay conditions.

Western blot

Polyclonal antibodies were produced in rabbits immunised with the PLA2 peptide sequence: NPYTHGYHQTCDKSTK (Inbiolabs, Tallin, Estonia). Samples were resolved by denaturing SDS-PAGE using 12 % polyacrylamide gels (BioRad, Hercules, CA, USA) and transferred to a polyvinylidene fluoride membrane (Millipore, Temecula, CA, USA). The membrane was blocked with 3 % non-fat milk in TPBS (PBS, 0·1 % Tween 20, pH 7·4) for 1 h, rinsed with TPBS and subsequently incubated with the primary antibody. Membranes were probed with primary anti-PLA2 rabbit (dilution: 1:2000) overnight at 4°C. Membranes were then washed four times for 10 min each with TPBS, incubated for 1 h with the secondary anti-rabbit horse radish peroxidase conjugated (1:2000; Dako, Glostrup, Denmark) in blocking buffer. Membranes were then treated with ECL Plus Western Blotting Detection Reagents (GE Healthcare, Piscataway, NJ, USA) for 5 min and photographed on hyperfilm (GE Healthcare) in the dark. The negatives were scanned and the area of sPLA2 IB protein bands was estimated using ImageJ software (http://rsb.info.nih.gov).

Open reading frame, alignments and statistics

Open reading frame sPLA2 IB for Atlantic cod was generated with Baylor College of Medicine HGSC Search Launcher (http://searchlauncher.bcm.tmc.edu/cgi-bin/seq-util/sixframe.pl). Alignments were done in ClustalW2 (http://www.ebi.ac.uk/Tools/clustalw2/index.html). Potential differences were tested with one-way ANOVA. Newman–Keuls post hoc test was used to test for significant differences between group means in an ANOVA. Correlations were tested with multiple regression analysis. Differences and effects were considered significant at P < 0·05 for all tests and differences were annotated with different letters in figures. ANOVA and post hoc analyses were performed on Statistica 9.0 (StatSoft, Inc., Tulsa, OK, USA).

Results

Larvae growth

Specific growth rate increased from 6·0 % at 10 dph to peak at 11·9 % at 34 dph when the SL was 7·75 mm. From 34 dph, there was a steady decrease in specific growth rate to 7·1 % at 97 dph. To evaluate the growth performance of fish larvae used in the present study with potential growth in wild cod, a size- and temperature-based growth model by Folkvord(Reference Folkvord15) was used:

T is temperature (°C) while DW is the dry weight (mg) of larvae at the first sampling point (3 dph). Dry weights were calculated based on SL according to the following equations from Finn et al. (Reference Finn, Ronnestad and van der Meeren14):

There were an increase in the difference between the observed length growth (SL) and modelled growth throughout the ontogeny series. The increase in percent difference between the modelled and observed growth had a slope of 0·7 (y = 0·6859x − 6·026, R 2 0·95); consequently, the fish were 61·02 mm at 97 dph, whereas the model predicted a SL of 95·86 mm, a difference of 57 % (Fig. 2).

Fig. 2 Size at sampling. Standard length (SL) of Atlantic cod larvae at sampling points analysed (mean values with their standard errors). The curve gives the predicted growth based on the model: SGR = 1·08+(1·79T )-0·074 × T (ln (DW)) − 0·0965 × T (ln DW)+0·0112 × T (ln DW)3(Reference Folkvord15). The model is based on data from wild populations. There was a significant increase in SL from 20 days post hatch (dph) on (one-way ANOVA, P < 0·05). SGR, Specific growth rate; DW, dry weight.

Identification of the secretory pancreatic phospholipase A2 IB gene

The expressed sequence tag (EST): EX726814 contained an open reading frame corresponding to a predicted amino acid sequence of matching sPLA2 group IB (Fig. 3). Atlantic cod open reading frame similar to sPLA2 group IB was aligned to sequences annotated to the PLA2 superfamily of D. labrax (CAA10765), P. major (BAA23737) and Fundulus heteroclitus (AAU50527). Sequences of Danio rerio (AAI14294), Sus scrofa (NP_001004037), Rattus norvegicus (NP_113773) as well as Homo sapiens (NP_000919) annotated to sPLA2 group IB were also aligned. To demonstrate that the previously listed sequences had the pancreatic loop unique to IB sPLAs, group V and X sPLAs were included in the alignment: H. sapiens (AAG43522) and Mus musculus (NP_001116426) from group V and H. sapiens (AAH69539), M. musculus (AAG43522) and D. rerio (NP_001002350) from group X. The Ca2+-binding loop (YGXXCGXGG) and the catalytic site (DXCCXXH) were conserved between all sequences aligned.

Fig. 3 Open reading frame based on EST (EX726814) from Atlantic cod. http://searchlauncher.bcm.tmc.edu/seq-util/Options/sixframe.html. Sequences for the Ca-binding loop(Reference Radunzneto, Corraze and Charlon2), the catalytic domain of the enzyme(Reference Radunzneto, Corraze and Charlon2), the pancreatic loop(Reference Geurden, Coutteau, Sorgeloos, Lavens and Jaspers3), epitope sequence used for antibody production (hatched box) and primers used for quantitative PCR (grey boxes).

Assay verification

Atlantic cod sPLA2 IB mRNA expression was assessed by RT-quantitative PCR in GI-tract, including pancreas, and also in the intestine, muscle, liver, gill, kidney and brain. The RT-PCR was run twenty-six and thirty-five cycles. After thirty-five cycles, all tissues except muscle produced a product when run on an ethidium bromide gel (data not shown). When the PCR was run twenty-six cycles, only GI-tract containing pancreatic tissue showed a band; all other tissues were blank (Fig. 4(a)). Ubiquitin was used as reference(Reference Olsvik, Softeland and Lie19, Reference Saele, Nordgreen and Hamre20). An increase from twenty-six to thirty-five PCR cycles gives a difference in amplification by the power of seven (Y = x 7).

Fig. 4 (a) PCR of secretory phospholipase A2 (sPLA2) IB primers on mRNA from gastrointestinal tract (GI-tract) with attached pancreatic tissue, intestine, muscle, liver, gill, kidney and brain of adult cod. (b) Western blot with rabbit anti-sPLA2 IB polyclonal antibody on homogenates of GI-tract. Only one band at 14 kDa was detected. (c) sPLA2 activity in liver, brain, kidney, gill and muscle tissue. Activity could be detected in all tissues except muscle. n.d., Not detected.

Western blot of GI-tract homogenates showed only one band with the approximate size of 14 kDa (Fig. 4(b)). Enzymatic activity was tested in tissues of adult Atlantic cod. Activity was detected in liver and brain (mean 0·27 (sd 0·05) μmol/min per ml) as well as in kidney and gill (mean 0·43 (sd 0·14) μmol/min per ml), but no activity was detected in skeletal muscle (Fig. 4(c)).

Ontogeny of secretory pancreatic phospholipase A2 group IB

The relative gene expression of PLA2 (quantitative RT-PCR) in homogenates of whole larvae was very low at the start of feeding (3 dph) until 48 dph, ranging from 0·0004 (sd 0·0002) to 0·04 (sd 0·01), respectively. There was a significant increase at 62 dph to 0·17 (sd 0·11). In GI-tract homogenates, there was significant increases from 0·0003 (sd 0·0001) at 34 dph to 0·586 (sd 0·192) at 62 dph when it plateaued (Fig. 5(A)).

Fig. 5 Secretory phospholipase A2 (sPLA2) IB expression in whole Atlantic cod () and Atlantic cod gastrointestinal tracts () at age 3 until 97 days post hatch (dph). (A) Mean normalised expression (MNE) of sPLA2 IB mRNA (quantitative RT-PCR). (B) Relative quantity of protein (Western blot). (C) Enzyme activity. a,b,c Mean values with unlike superscript letters were significantly different (one-way ANOVA, P < 0·05); analysis of whole larvae homogenates and gastrointestinal tracts homogenates were not tested against each other.

Protein expression was not detectable in whole fish homogenates until 62 dph. In GI-tract homogenates, there was an increase in protein expression from 48 to 62 dph and then again from 83 to 97 dph (Fig. 5(B)). There was a significant correlation between mRNA expression and protein expression both in larvae homogenates (P < 0·0001, r 2 0·9) and in GI-tract (P = 0·004, r 2 0·5) (Fig. 6).

Fig. 6 Correlation between mRNA expression and protein expression of secretory phospholipase A2 (sPLA2) IB in gastrointestinal tract homogenates; y = 0·086+0·0002 × x, P = 0·0039, r 2 0·51. MNE, mean normalised expression.

Enzymatic activity was detectable already from first exogenous feeding. Homogenates of whole larvae had an sPLA2 activity of 0·70 μmol/min per g from 3 to 20 dph. At 34 dph, the activity decreased to 0·36 (sd 0·04) μmol/min per g. There was no increase in activity from 34 to 62 dph in larvae homogenates. The activity in GI-tract homogenates was stable from 34 to 97 dph, with an average activity of 1·11 (sd 0·18) μmol/min per g (Fig. 5(C)). Enzymatic activity did not correlate with mRNA nor with protein expression.

Gastrointestinal-tract v. body secretory phospholipase A2 specific activity

Average wet weights of the larvae at ages 34, 48 and 62 dph were 8·18, 34·9 and 146 mg, respectively. The dissected GI-tracts weighed 1·51, 2·21 and 9·49 mg at the same ages. Consequently, the GI-tract made up 18·5, 9·19 and 6·48 % of the total body wet weight at 34, 48 and 62 dph, respectively. The average enzymatic activities at age 34, 48 and 62 dph were 0·0030, 0·014 and 0·064 μmol/min per fish, respectively. Average activities in dissected GI-tracts were 0·0019, 0·0043 and 0·0092 μmol/min per GI-tract. Hence, the activity of the GI-tract contributed with 63·2, 30·8 and 14·2 % of the total body enzyme activity at 34, 48 and 62 dph, respectively (Fig. 7).

Fig. 7 The secretory phospholipase A2 activity in whole Atlantic cod larvae () and their gastrointestinal (GI)-tract (). Inset shows correlation between percent size of GI-tract of whole larvae and percent activity in GI-tract to activity in whole larvae at ages 34, 48 and 62 d post hatch (dph).

Discussion

The growth rate of cod larvae when fed natural zooplankton can be very high and is reported to range from 13 to 30 %/d during the first 50 d(Reference Finn, Ronnestad and van der Meeren14Reference Otterlei, Nyhammer and Folkvord21). Atlantic cod larvae fed live feed-like enriched rotifers (B. plicatilis) and Artemia and formulated diets generally have poor growth compared with those fed wild collected zooplankton(Reference Busch, Falk-Petersen and Peruzzi22). For example, cod larvae fed Artemia and formulated feed had a growth rate ranging from 5·1 to 10·7 % between 22 and 64 dph(Reference MacQueen Leifson, Homme and Lie23, Reference Callan, Jordaan and Kling24). Fish in the present study grew well compared with those in previous experiments evaluated using the same growth model(Reference Folkvord15), by Busch et al. (Reference Busch, Falk-Petersen and Peruzzi22). The fish in the present study were 13·5 and 31·7 % shorter than the modelled predictions at 9·9 mm SL (34 dph) and 23·8 mm SL (62 dph), respectively, while in another trial with a similar diet to that used in the present experiment, the larvae were 43·9 and 42·0 % shorter than the model at a similar SL(Reference Callan, Jordaan and Kling24). We may therefore conclude that the ontogeny series of cod larvae analysed in the present study had good growth compared with other intensive rearing trials where larvae were start fed on rotifers and weaned at an early stage.

The family of sPLA2 consists of the groups I, III, V and X, containing all together ten enzyme forms as described in mammals. The sPLA2 IB belongs to a family of ten sPLA2 that share a highly conserved region for a Ca2+-binding loop (XCGXGG) and a catalytic site (DXCCXXH)(Reference Murakami and Kudo9). These sites are conserved between Atlantic cod and the evaluated fish, D. labrax, P. major, D. rerio and F. heteroclitus as well as in the mammals S. scrofa, R. norvegicus and H. sapiens. However, in front of the Ca2+ loop, there is also a conserved region of the amino acids tyrosine (Y), glycine (G) and cysteine (C) between all listed species in Fig. 8, with the exception of Atlantic cod that has a tryptophan (W) in place of the C. The codon for C is UGU or UGC and for W it is UGG. Since C domains are much conserved(Reference Sevier and Kaiser25), it is likely that the third G in the codon is a sequencing error and should in fact be a U or a C. With this exception, all C domains are conserved between the fishes listed in Fig. 8.

Fig. 8 Alignment of the open reading frame amino acid sequences of phospholipase A2 with the known pancreatic PLA2 fish sequences: Dicentrarchus labrax (CAA10765), Pagrus major (BAA23737), Fundulus heteroclitus (AAU50527), Danio rerio (XP_700448) and the secretory PL A2 (sPLA2) IB mammalian sequences: Sus scrofa (NP_001004037), H. sapiens (NP_000919) and R. norvegicus (NP_113773). For visualisation of characteristics of the pancreatic form of sPLA2, sequences of the group V sPLA2: M. musculus (EDL13282) and H. sapiens (AAG43522) and the group X sPLA2: M. musculus (NP_001116426), Homo sapiens (AAH69539) and D. rerio (NP_001002350) were included in the alignment. Accession numbers are given in parenthesis. Sequences for the Ca-binding loop (1), the catalytic domain of the enzyme (2), the pancreatic loop (3). *Indicates conserved amino acid residues identical to those of Atlantic cod, –indicates amino acid residues absent in the sPLA2 groups V and X.

Distinctive for the pancreatic form sPLA2 group IB involved in PL digestion is the pancreatic loop containing the domain PYTXX. This domain is conserved between all listed sPLA2 with the exception of enzyme groups V and X and the F. heteroclitus sequence (Fig. 8). The sPLA2 group V and X are not expressed in pancreatic tissue and are not involved in PL digestion(Reference Triggiani, Granata and Giannattasio26). We may therefore conclude that the evaluated sequence in Atlantic cod most likely encodes for sPLA2 IB. Further supporting this, the protein weight of sPLA2 IB has previously been reported as 14 kDa(Reference Murakami and Kudo9Reference Schaloske and Dennis29), which was the size of the protein picked up by our antibody. In addition, we also provide proof that the PLA2 sequences from D. labrax and P. major probably should be annotated sPLA2 IB.

The primers used in the present study may amplify PLA2 isoforms present in other tissues than in the pancreatic tissue. Iijima et al. (Reference Iijima, Uchiyama and Fujikawa27) characterised three isoforms of group I sPLA2 in the gills of red sea bream, out of which one belonged to group IB. It is plausible that there are similar isoforms in Atlantic cod. The sPLA2 IB has also been found in trace amounts in other organs, such as lung, kidney and spleen, in rat(Reference Murakami and Kudo9Reference Tojo, Ono and Kuramitsu28). In the present study, mRNA expression of sPLA2 IB in pancreas containing tissue was at least to the seventh power higher than in the liver, brain, kidney and gill. It is therefore likely that relative quantities of mRNA measured in GI-tract system as well as in whole larvae reflect the pancreatic production.

The enzyme activity assay used in the present study was specific for secretory enzyme forms, but cannot differentiate between different groups of sPLA2. Analysing the homogenates of whole organisms and organ systems such as the GI-tract will therefore include the catalytic capability of PL sn-2 fatty acid hydrolysis of many tissues and enzyme isoforms(Reference Hendrickson, Hendrickson and Dybvig10, Reference Reynolds, Hughes and Dennis11). Iijima et al. (Reference Iijima, Uchiyama and Fujikawa27) found that the PLA2 activity in the gills of red sea bream was seventy times higher than in the pancreatic tissue. In the present study, the activity in gill tissue of juvenile cod was the same as in kidney but less than half of the activity found in the GI-tract homogenate that included pancreatic tissue and gut content. Nevertheless, there is no doubt that enzyme activity data presented here and in other papers(Reference Ozkizilcik, Chu and Place30) represent the activity of a cocktail of PLA2 types from various tissues. There have been attempts to minimise this problem. For example, Cahu et al. (Reference Cahu, Infante and Takeuchi7) divided the larvae in segments, but the pancreas segment probably still included the parts of kidney and liver, the important contributors to PLA2 activity.

The mRNA expression of sPLA2 IB in whole fish was stable but low at the start of feeding, but increased from 48 dph and 15·1 mm SL, and was higher again at 62 dph and 23·8 mm SL. Uematsu et al. (Reference Uematsu, Kitano and Morita13) did not find a sPLA2 IB immunohistochemical signal until 13 dph in pancreatic acinar cells from red sea bream, which is 11–9 d post first exogenous feeding(Reference Nguyen, Satoh and Haga31). The intensity of staining then increased steadily during development. In the present study, sPLA2 IB Western blots of homogenates from larvae did not pick up any signal until 62 dph. This together with the findings of Uematsu et al. (Reference Uematsu, Kitano and Morita13) demonstrates that the quantity of sPLA2 IB is under the detection limit of these assays and therefore quite low during the early larval stages of both red sea bream and Atlantic cod. However, Ozkizilcik et al. (Reference Ozkizilcik, Chu and Place30) measured PLA2 activity on whole eggs and larvae of striped bass (Morone saxatilis) and found a steady increase in activity from fertilisation until the juvenile stage. As emphasised by the authors, activity assays register all types of PLA2 activity and are unsuitable for assessment of isoform-specific activity during development. This is further emphasised by the elevated PLA2 activities in starved larvae when compared with fed larvae(Reference Ozkizilcik, Chu and Place30). An important difference between the present data and those of Ozkizilcik et al. (Reference Ozkizilcik, Chu and Place30) is that while they analysed larvae with empty guts, we analysed larvae with filled guts. The latter would then include any sPLA2 activity of ingested rotifers in addition to increased enzymatic activity of the larvae. This is visualised by the significant drop in whole larvae sPLA2 activity after 20 dph when weaning of larvae onto the formulated diet began (Fig. 5(C)). This drop is probably due to the absence of rotifer enzyme activity and not the decreased production of sPLA2 since it is only seen in activity and not in mRNA status (Fig. 5). According to Infante & Cahu(Reference Infante and Cahu32), the levels of PL in the diet regulate sPLA2 mRNA in D. labrax larvae. However, no such regulation was apparent in cod from the present trial. The formulated diet contained 14–15 % total lipid of DM of which 80–86 % was PL (Gemma micro), whereas the rotifers fed had a total lipid content of 8·5 (sd 1·8)% of DM of which 37 (sd 3)% is PL(Reference Hamre, Mollan and Saele33). Hence, when the larvae are weaned, they change from a low PL diet of 3·15 % to a high PL diet of 12 % of dry weight. Instead of up-regulating the sPLA2 IB production and sPLA2 activity to accommodate for the increase in dietary PL, the enzyme production is unaffected and the enzymatic activity is decreased.

There was a linear correlation between the mRNA expression and the protein expression in GI-tract homogenates, with a coefficient of determination of 0·51 (Fig. 6). The mRNA of sPLA2 IB is only found in pancreatic acinar cells, whereas the protein would be present in the intestinal lumen as well in the pancreas(Reference Murakami and Kudo9). The remaining 49 % of the variation between the quantity of mRNA and protein can therefore be explained by post-transcriptional regulations of protein synthesis and by enzyme present in the gut lumen.

In Atlantic cod, we found a close relationship between the ratio of GI-tract to whole larvae wet weight and the ratio of GI-tract to total larvae enzyme activity. In turbot larvae, 61 % of the neutral lipolytic activity came from the gut at 12 dph decreasing to 52 % at 24 dph(Reference Hoehne-Reitan, Kjorsvik and Reitan34). This coincides with the trend shown in cod and is probably correlated with the decreasing proportion of the GI-tract to whole body mass during ontogeny.

A question that can be asked based on the present results is: what does the ontogeny of the digestive enzyme expression and activity tell us about the digestive capabilities of the fish larvae? The answer is that it appears to tell only part of the story, i.e. when the adult form of digestion develops. Fish larvae require PL-rich diets(Reference Cahu, Gisbert and Villeneuve6, Reference Tocher, Bendiksen and Campbell35) and it has been demonstrated that intact PL is absorbed in intestinal epithelium in larval zebrafish(Reference Carten and Farber36, Reference Farber, Pack and Ho37). We propose that in the early larval stages, the endogenous production of sPLA2 IB is low and exogenous enzyme contribution from live prey is important for PL digestion in addition to the ability of the larvae to absorb intact PL. During ontogeny, these mechanisms may disappear and/or become less important in parallel with an increase in the endogenous enzyme production as the fish acquire the adult digestion form.

Acknowledgements

We thank Line Muklebust for valuable help with Western blots and Tina Constanse Rosvold for valuable help during the tedious sampling and dissection of GI-tracts. We also thank Samuel James Penglase for painstaking correction of the manuscript and for the valuable inputs. We thank Marine Harvest Cod AS. This work is a part of the project financed by the Research Council of Norway: ontogeny of lipid digestion and the effects of feeding pre-digested lipids to Atlantic cod (G. morhua) larvae 179016/S40. There are no conflicts of interest. A. N. was responsible for sampling and RNA extraction. P. A. O. identified sPLA2 IB in Atlantic cod and designed quantitative PCR primers. Ø. S. performed the mRNA, protein, enzyme and bioinformatics analysis. K. H. planned the study and was the project leader, and together with Ø. S., he is the major author of the manuscript. All the authors contributed to writing the manuscript.

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Figure 0

Fig. 1 Trial and sampling scheme. The arrow gives the type of diet during the sampling period, numbered circles indicate the number of pooled individuals in each sampling and the age of larvae at sampling is given in days post hatch (dph). GI, gastrointestinal tract.

Figure 1

Fig. 2 Size at sampling. Standard length (SL) of Atlantic cod larvae at sampling points analysed (mean values with their standard errors). The curve gives the predicted growth based on the model: SGR = 1·08+(1·79T )-0·074 × T (ln (DW)) − 0·0965 × T (ln DW)+0·0112 × T (ln DW)3(15). The model is based on data from wild populations. There was a significant increase in SL from 20 days post hatch (dph) on (one-way ANOVA, P < 0·05). SGR, Specific growth rate; DW, dry weight.

Figure 2

Fig. 3 Open reading frame based on EST (EX726814) from Atlantic cod. http://searchlauncher.bcm.tmc.edu/seq-util/Options/sixframe.html. Sequences for the Ca-binding loop(2), the catalytic domain of the enzyme(2), the pancreatic loop(3), epitope sequence used for antibody production (hatched box) and primers used for quantitative PCR (grey boxes).

Figure 3

Fig. 4 (a) PCR of secretory phospholipase A2 (sPLA2) IB primers on mRNA from gastrointestinal tract (GI-tract) with attached pancreatic tissue, intestine, muscle, liver, gill, kidney and brain of adult cod. (b) Western blot with rabbit anti-sPLA2 IB polyclonal antibody on homogenates of GI-tract. Only one band at 14 kDa was detected. (c) sPLA2 activity in liver, brain, kidney, gill and muscle tissue. Activity could be detected in all tissues except muscle. n.d., Not detected.

Figure 4

Fig. 5 Secretory phospholipase A2 (sPLA2) IB expression in whole Atlantic cod () and Atlantic cod gastrointestinal tracts () at age 3 until 97 days post hatch (dph). (A) Mean normalised expression (MNE) of sPLA2 IB mRNA (quantitative RT-PCR). (B) Relative quantity of protein (Western blot). (C) Enzyme activity. a,b,c Mean values with unlike superscript letters were significantly different (one-way ANOVA, P < 0·05); analysis of whole larvae homogenates and gastrointestinal tracts homogenates were not tested against each other.

Figure 5

Fig. 6 Correlation between mRNA expression and protein expression of secretory phospholipase A2 (sPLA2) IB in gastrointestinal tract homogenates; y = 0·086+0·0002 × x, P = 0·0039, r2 0·51. MNE, mean normalised expression.

Figure 6

Fig. 7 The secretory phospholipase A2 activity in whole Atlantic cod larvae () and their gastrointestinal (GI)-tract (). Inset shows correlation between percent size of GI-tract of whole larvae and percent activity in GI-tract to activity in whole larvae at ages 34, 48 and 62 d post hatch (dph).

Figure 7

Fig. 8 Alignment of the open reading frame amino acid sequences of phospholipase A2 with the known pancreatic PLA2 fish sequences: Dicentrarchus labrax (CAA10765), Pagrus major (BAA23737), Fundulus heteroclitus (AAU50527), Danio rerio (XP_700448) and the secretory PL A2 (sPLA2) IB mammalian sequences: Sus scrofa (NP_001004037), H. sapiens (NP_000919) and R. norvegicus (NP_113773). For visualisation of characteristics of the pancreatic form of sPLA2, sequences of the group V sPLA2: M. musculus (EDL13282) and H. sapiens (AAG43522) and the group X sPLA2: M. musculus (NP_001116426), Homo sapiens (AAH69539) and D. rerio (NP_001002350) were included in the alignment. Accession numbers are given in parenthesis. Sequences for the Ca-binding loop (1), the catalytic domain of the enzyme (2), the pancreatic loop (3). *Indicates conserved amino acid residues identical to those of Atlantic cod, –indicates amino acid residues absent in the sPLA2 groups V and X.