What this is
- The study investigates the role of oxytocin/vasopressin-like peptides in the of the mud crab Scylla paramamosain.
- It identifies the expression patterns of related genes and their potential inhibitory effects on ovarian development.
- The findings suggest that the oxytocin/vasopressin signaling system may regulate reproductive processes through neuroendocrine mechanisms.
Essence
- Oxytocin/vasopressin-like peptides may inhibit in mud crabs by reducing estrogen levels and affecting gene expression in reproductive tissues.
Key takeaways
- Oxytocin/vasopressin-like peptides are expressed in various tissues, including the ovary and hepatopancreas, indicating their potential role in reproductive regulation.
- In vitro and in vivo experiments show that synthetic oxytocin/vasopressin-like peptides significantly reduce the expression of -related genes and estrogen levels.
- The study suggests that the oxytocin/vasopressin signaling system may act through neuroendocrine and autocrine mechanisms to inhibit ovarian development in mud crabs.
Caveats
- The exact molecular mechanisms by which oxytocin/vasopressin-like peptides inhibit remain unclear, requiring further investigation.
- The study primarily focuses on gene expression levels and does not provide direct evidence of functional changes in reproductive outcomes.
Definitions
- Vitellogenesis: The process of yolk formation and accumulation in oocytes, essential for embryo development.
AI simplified
1. Introduction
Oxytocin (OT) and vasopressin (VP), the most ancient neuropeptides, were discovered from mammalian posterior pituitary in the early 1920s, having the oxytocic action or causing an increase in blood pressure [1]. Subsequently, they were purified and sequenced in 1953 before any other neuropeptides, and their preprohormones were firstly cloned from a rat genomic library in the early 1980s [2,3,4].
In mammals, the genes of OT and VP lie in the same chromosome towards each other, possessing a highly similar structure: a nonapeptide, located after a signal peptide and followed by a dibasic cleavage site and a neurophysin. The two nonapeptides both display a ring-like structure with an intramolecular disulfide bond (Cys1–Cys6), discriminated at position 8 where there is a neutral amino acid for OT, but a basic for VP [5,6]. And the neurophysin, with 14 cysteine residues, is an OT/VP-carrier protein which is essential to fold and sort the prohormones [7]. OT and VP are synthesised by the neurosecretory cells of supraoptic and paraventricular nucleus in hypothalamus and transported to the posterior pituitary via axons for secretion, which are multifunctional with essential roles in the regulation of social and reproductive behavior [8,9]. OT is mainly involved in inducing uterine contraction during parturition and milk ejection during lactation, and affecting parental care, social cognition, learning and memory [9,10,11], while VP is related to parental care, male/female pair bonding, blood pressure control and antidiuretic actions by stimulating water reabsorption via the renal collecting ducts [12]. The functions of OT/VP are mediated by the four receptors belonging to a family of G protein-coupled receptors (OTR, V1aR, V1bR and V2R) [13]. Among them, OTR, V1aR and V1bR all couple to the inositol trisphosphate (IP3)/Ca2+ signal transduction pathway, while V2R regulates the level of intracellular cAMP by the coupled adenylate cyclase [14,15,16,17]. Besides, OT/VP signaling system has also been reported in a number of other vertebrates such as birds, reptiles, amphibians and fishes, which all are supposed to have evolved from vasotocin, the ancestral nonapeptide, by gene duplication [18].
In invertebrates, OT or VP-like peptide has been widely identified among various phyla, while the co-occurrence of the two in the same species had never been demonstrated. In crustaceans, the OT/VP-like peptides have been reported in the blue swimming crab Portunus pelagicus, the water flea Daphnia pulex, the giant freshwater prawn Macrobrachium rosenbergii and the mud crab Scylla paramamosain, but lack of function tests [19,20,21,22]. Though the functional expression in cells and characterisation of OT/VP-like receptor have been investigated in mollusks, insects and nematodes, so far it isn’t studied in crustaceans [20,23,24,25].
In oviparous animals, the vitellogenesis, divided into autosynthesis and heterosynthesis according to the yolk origins, is an important process for the formation and accumulation of various yolk substances, which can provide nutrients and energy for the development of embryos and early larvae [26]. In crustaceans, the regulation on the ovarian maturation involves many neuropeptides. In the classic Panouse experiment in 1944, the removal of eyestalk in the shrimp Palaemon serratus resulted in enlarged ovaries and precocious eggs, suggesting that the effect was due to the removal of vitellogenesis-inhibiting hormone (VIH). Then it was isolated from the eyestalk of the American lobster Homarus americanus firstly and demonstrated to inhibit vitellogenesis [27,28]. Recently, crustacean female sex hormone (CFSH), isolated from the sinus gland of the blue crab Callinectes sapidus, is considered to be the female sex-determining hormone [29]. Besides in S. paramamosain, the red-pigment concentrating hormone (RPCH), secreted from the eyestalk ganglion, stimulates ovarian development, while the short neuropeptide F (sNPF) and allatostatin-C show inhibitory effect on ovarian development [30,31]. In P. pelagicus, it was reported that the PpOT/VP-like peptide could inhibit the release of steroid hormones (17β-estradiol and progesterone) in ovarian explants in vitro [19]. Up to now, the molecular mechanism of OT/VP-like peptides on crustacean reproduction is unclear.
In this study, Spot/vp and Spot/vpr-like gene sequences were cloned from S. paramamosain, the tissue distribution and expression profiles during vitellogenesis were detected. Moreover, in vivo and in vitro experiments were performed to explore the role of the signaling system in vitellogenesis.
2. Results
2.1. Molecular Cloning and Bioinformatics of SpOT/VP-Like Preprohormone
The full-length sequence of Spot/vp-like (GenBank accession: MT123288↗) cDNA is 853 bp with 63 bp 5′ untranslated region (UTR), 313 bp 3′ UTR and 477 bp open reading frame (ORF). The preprohormone is composed of 158 amino acids containing a nonapeptide with the structure CFITNCPPGamide, which is located after a signal sequence and followed by a dibasic cleavage sites (GKR) and a neurophysin. The nonapeptide has a predicted molecular weight of 951.12 Da and a theoretical isoelectric point of 5.51, and the neurophysin has 14 cysteine residues (Figure A1A). Multiple sequence alignment suggests that the nonapeptides and three rigid cage-like domains are highly conserved: a neuropeptide-containing domain (one disulfide bonds) and two neurophysin domains (one four and the other three disulfide bonds) (Figure 1). Phylogenetic analysis show that SpOT/VP-like preprohormone is clustered into the branch of crustaceans, then the branch with mollusks before insects (Figure A2).
2.2. Molecular Cloning and Bioinformatics of SpOT/VPR-Like Preprohormone
The Spot/vpr-like (GenBank accession: MT123289↗) cDNA ORF sequence is 1308 bp encoding 435 amino acids, which contains seven α-helical transmembrane (TM) regions with a predicted molecular weight of 48,067.19 Da and a theoretical isoelectric point of 7.01. The N-terminal domain is in the extracellular with two sites of N-linked glycosylation (Asn-X-Ser/Thr) and the C-terminal is in the intracellular. The preprohormone also contains some consensus sequences sites about phosphorylation for protein kinase C (Ser/Thr-X-Arg/Lys), casein kinase II (Ser/Thr-X-X-Asp/Glu) and cAMP-dependent protein kinase (Arg/Lys-Arg/Lys-X-Ser/Thr) (Figure A3) [32]. Multiple sequence alignment suggests that, except TM regions, the first and second extracellular loops, between TM2 and TM3 and between TM4 and TM5 respectively, have the highest homology, while the third intracellular loop shows hardly any sequence identity, in which SpOT/VPR-like preprohormone contains ~20 amino acids more than vertebrate receptors (Figure 2).
2.3. Expression Profiles of Spot/vp and Spot/vpr-Like mRNA
RT-PCR shows that Spot/vp-like transcripts highly expressed in the nervous tissues, midgut, gill and epidermis, less express in the hepatopancreas and ovary, and hardly detected in the others. Spot/vpr-like are widespread in various tissues including the hepatopancreas, ovary and hemocytes (Figure 3A). qRT-PCR shows that there is a consistent temporal expression profile between Spot/vp-like transcripts in the nervous tissues and ovary and Spot/vpr-like in the ovary: highest expression level at pre-vitellogenic stage, significantly down-regulated at early and maintained lower at late (Figure 3B,C).
2.4. In Situ Hybridisation of Spot/vp and Spot/vpr-Like mRNA
The Spot/vp-like mRNA is mainly detected in 6th, 7th clusters of protocerebrum and 8th, 9th of deutocerebrum, and both in the oocytes and follicular cells of ovary (Figure 4A–I). The Spot/vpr-like is mainly localised in the F-cells of hepatopancreas and the oocytes in the ovary (Figure 4J–O). All control sections, probed with sense strand RNA, show no positive signal.
2.5. Synthetic SpOT/VP-Like Peptide Treatment In Vitro
In the hepatopancreas cultured in vitro, the mRNA expression level of Spvg is significantly down-regulated at 12 h with 10−7 M synthetic peptide administration (p < 0.05) (Figure 5A). The levels of E2 in the media is significantly decreased at 6 h, 10−8 M treatment and 12 h, 10−7 and 10−8 M treatments, respectively (p < 0.05), and extremely significantly declined at 12 h, 10−6 M treatment (p < 0.01) (Figure 5B). In the ovary, the mRNA expression level of Spvgr is extremely significantly down-regulated at 12 h, 10−9 M treatment (p < 0.01) (Figure 5C). The levels of E2 in the media is highly significantly lower at 6 h, 10−9 M treatment (p < 0.01), and significantly declined at 12 h, 10−9 M treatment, respectively (p < 0.05) (Figure 5D).
2.6. Synthetic SpOT/VP-Like Peptide Treatment In Vivo
The mRNA expression level of Spvg in the hepatopancreas and the E2 content in haemolymph are significantly down-regulated after the injection of synthetic peptide (p < 0.05) (Figure 6A,C). The mRNA expression levels of Spvg and Spvgr in the ovary were both not decreased significantly, but showed the inhibitory trends (Figure 6B). The oocyte diameter in the peptide injection group (52.8 ± 3.96 μm) was significantly shorter than that in crustacean physiological saline (CPS) group (74.6 ± 5.18 μm) (Figure 6D–G).
2.7. RNA Interference in the Hepatopancreas Explants In Vitro
In the hepatopancreas explants, the mRNA expression level of Spot/vpr was significantly down-regulated after the RNA interference (p < 0.05) (Figure 7A); simultaneously, the mRNA expression level of Spvg was significantly up-regulated with the treatment of synthetic peptide after RNA interference (p < 0.05) (Figure 7B).
3. Discussion
Hitherto, the study of OT/VP-like signaling system in crustacean reproduction has been rarely reported. In this study, it is suggested that the signaling system can inhibit vitellogenesis by means of neuroendocrine and autocrine/paracrine in S. paramamosain.
SpOT/VP-like precursor sequence is more than 60% similar to those of other crustaceans such as Portunus pelagicus (GenBank accession: AUT12056.1↗) and Penaeus vannamei (GenBank accession: ROT67110.1↗). The molecular structure of the nonapeptides is highly conserved in various phyla, which makes it more universal to induce the functional response resulted from heterogenous OT/VPs. The bioactivity, resulted from Conus arg-conopressin-g/s in the brain of rat, is similar to those induced by vertebrate OT/VPs [33]. And the OT-like peptide from the pufferfish Fugu rubripes can functionally express in rat nerve cells [34]. Therefore, the discovery and functional screening of natural OT/VP peptides is an effective strategy for ligand selection and drug discovery, targeting at human OT/VP receptors [35]. OT/VP-like precursors in crustaceans clustered with those in mollusks firstly, then insects which belong to the same clade Pancrustacea. The strange result may be because that crustaceans are more closely related to the common ancestor of arthropods than insects in evolutionary status, such as D. pulex, considered to be the ancestor of insects with the divergence in ~420 million years ago [36]. Moreover, in order to adapt to a variety of environments during the evolution process from aquatic to terrestrial taxa, structures and functions of arthropods evolve over time. The OT/VP signaling system, lasting to crustaceans, is lost at least twice in insects which had been replaced by AKH, CCAP or Corazonin hormone systems, all participating in osmotic regulation and metabolism etc. [20].
The SpOT/VPR-like is a G-protein coupled receptor with seven α-helical transmembrane regions. Except TMs regions, the first and second extracellular loops are the most conserved regions, connected by a disulfide bonds and important in ligand binding [37]. The sites of N-linked glycosylation in the extracellular N-terminal domain contribute to the target to plasma membrane, and the consensus sequences sites about phosphorylation are important in the modulation of G protein coupling and receptor function [32]. Compared with OT, SpOT/VPR-like sequence is more similar to V1aR in mammals such as the mouse Mus musculus (GenBank accession: NP_058543.2↗) and the domestic horse Equus caballus (GenBank accession: XP_001917958.4↗) with homologies over 40%, suggesting that it may be a VP-like receptor. And when synthetic SpOT/VP was added after knocking down Spot/vpr in vitro, the inhibitory effect of synthetic peptide was relieved, indicating that the receptor was SpOT/VPR-like to some extent. It is the first time to clone and characterise OT/VPR-like in crustaceans. There are usually two sets of OT/VP signaling systems in molluscs, probably due to the additional gene replication [9,25]. Similarly, two OT/VP-like receptor (GenBank accession: ROT66533.1↗; XP_027226674.1↗) sequences, found in the genomic database of P. vannamei, suggested that multiple OT/VP signaling systems may also exist in crustaceans.
Spot/vp-like mRNA transcripts are mainly expressed in the nervous system, which is similar to the immunohistochemical results of invertebrates such as the hydrozoan Hydra magnipapillata and the polychaete Neanthes japonica, and the in situ hybridisation outcomes in the ant Camponotus fellah and the octopuses Octopus vulgaris [38,39,40,41,42]. The transcripts are also highly expressed in the midgut and gill, having the same expression pattern to Ppot/vp-like mRNA transcripts in P. pelagicus [19]. It is suggested that SpOT/VP-like peptide can be involved in osmotic regulation, which is probably induced via crustacean hyperglycaemic hormone (CHH) as reported in the crab Pachygrapsus marmoratus and the crayfish Astacus leptodactylus [43,44]. Spot/vpr-like mRNA transcripts are expressed in various tissues, suggesting that SpOT/VP signaling system is pleiotropic, similar to Lys-CP (from Lymnaea stagnalis) and OP (from Octopus vulgaris) [24,25,42].
In situ hybridisation shows that Spot/vp-like mRNA, similar to mollusk op/ct, is distributed in various kinds of neurons in cerebral ganglion, such as 6th and 7th neuronal clusters involved in reproductive regulation, and 8th and 9th in olfaction, learning and memory regulation [45,46,47]. Spot/vpr-like mRNA is expressed in F-cells of hepatopancreas, the main sites of enzyme synthesis, suggesting that the system may participate in the regulation of hepatopancreas on digestion, metabolism and reproduction. Besides, at early vitellogenic stage, Spot/vp-like mRNA distributes in oocytes/follicular cells, while Spot/vpr-like distributes in oocytes, indicating that SpOT/VP-like from oocytes/follicular cells might act on oocytes. This result is different from the short neuropeptide F (sNPF) previously reported in the ovary in S. paramamosain, which showed that sNPF, synthesised by follicular cells, could act on oocytes/follicular cells [48]. Therefore, the communication might exist between oocytes and follicular cells in S. paramamosain, and we speculated that regulatory mode of autocrine/paracrine factors in the ovary is multifarious in crustaceans.
In mammals, both stimulatory and inhibitory effects of OT/VP/VTs on the release of E2/P4 (Progesterone), the vertebrate-type steroid hormones, from granulosa cells were reported [49,50,51]. Besides, in the catfish Heteropneustes fossilis, the vasotocin detected in granulosa cells of post-vitellogenic and absent in immature follicles, could promote the releases of E2, P4, P4 derivatives and prostaglandin, and cause the germinal vesicle breakdown and ovulation, which was suggested to correlate with the stage of luteinisation [52,53,54,55]. The E2 and P4-like were first discovered in crustaceans in 1978 [56]. Furthermore, the existence of E2/P4 in hepatopancreas, ovary and haemolymph, and the presence and activities of steroid-related enzymes (20α-HSD, 17β-HSD, 3β-HSD, 17β-HSD8) were recently reported in crustaceans, by which vitellogenesis was controlled [57,58,59,60,61,62]. Temporal expression profiles of Spot/vp and Spot/vpr-like mRNA showed that they might be involved in inhibiting ovarian development. Both in vitro cultured and in vivo long-term injection experiment showed that synthetic SpOT/VP-like peptide could significantly inhibit the expression of Spvg/Spvgr in the hepatopancreas/ovary, respectively, which could be achieved by inhibiting the release of 17β-estradiol (E2) from the hepatopancreas/ovary. Histological analysis further showed that ovarian development was suppressed after the injection of synthetic peptide, with the significantly subduced oocyte growth. And it is probably resulted from less synthesis of yolk substances, and lack of accumulation of yolk substances in oocytes. Similarly, in P. pelagicus, the synthetic PpOT/VP-like peptide also significantly inhibited the releases of E2 and P4 in the culture media from stage II and IV ovaries [19]. In conclusion, SpOT/VP-like signaling system might inhibit vitellogenesis as neuroendocrine and autocrine/paracrine factors by inhibiting the release of E2 in S. paramamosain. This paper has enriched the researches on the OT/VP signaling system and the effect of neuropeptides on reproductive regulation in crustaceans. However, the detailed mechanisms on ovarian development should be clarified with more experiments in the future.
4. Materials and Methods
4.1. Animals
The female S. paramamosain, purchased at No.8 fishery market, Xiamen, China, were kept in plastic tanks containing sea water with aeration for 6 h at 27.0 ± 2.0 °C (temperature) and 27.0 ± 0.5 ppm (salinity), and fed with fresh clam Ruditapes philippinarum. In S. paramamosain, vitellogenesis can be classified into three stages according to the previous study: pre-vitellogenic, early vitellogenic and late vitellogenic stage [63]. All animal procedures were carried out in strict compliance with the National Institute of Health Guidelines for the Care and Use of Laboratory Animals.
4.2. Molecular Cloning, Bioinformatics and Phylogenetics of SpOT/VP-Like Peptide and Its Receptor
Search for the nucleotide sequences of Spot/vp-like peptide and its receptor in the transcriptome of S. paramamosain cerebral ganglia, reported in previous studies, by BLAST against GenBank, non-redundant (Nr) and Gene Ontology (GO) [22]. The RNA, extracted from cerebral ganglia using Trizol reagent (Invitrogen, Carlsbad, CA, USA), was used for cDNA synthesis with the RevertAidTM First Strand cDNA Synthesis Kit (Fermentas Inc., Ontario, Canada) and 5′/3′ RACE-cDNA synthesis with the SMARTTM RACE cDNA Amplification Kit (TaKaRa, Shiga, Japan). The full sequence was cloned according to the user manual for the SMARTTM RACE 5′/3′ Kit. All PCR products, separated by 1.0% (w/v) agarose gel electrophoresis and purified using agarose gel purification and extraction kit (Aidlab, Beijing, China), were cloned into the pMD19-T vector (Promega, Madison, WI, USA) and sequenced by Sangon Biotechnology Company Limited (Shanghai, China). ORFs and amino acid sequences were predicted by DNAStar software, and protein composition, molecular weight and isoelectric point were analysed by ExPASy software. The preprohormone sequences of OT/VPs and OT/VPRs from S. paramamosain against other species were obtained from NCBI, which were used to create the multiple sequence alignment by MEGA 7.0 software. Phylogenetic trees were carried out via the neighbor-joining method with 1000 bootstrap replicates using MEGA 7.0 software. Moreover, signal peptides were predicted by SignalP 5.0, cleavage sites, post-translational modifications and bioactive peptide products were predicted by NeuroPred, and transmembrane domains were predicted by TMHMM tool. All primers are listed in Table A1.
4.3. Tissue Distributions of Spot/vp and Spot/vpr-Like mRNA
The RNAs (n = 3), extracted from eyestalk ganglion, cerebral ganglion, thoracic ganglion, hepatopancreas, ovary, midgut, heart, stomach, gill, muscle, epicdermis and hemocytes at early vitellogenesis stage, were used for cDNA synthesis. Semi-quantitative RT-PCR was performed to detect the tissues distributions of Spot/vp and Spot/vpr-like transcripts. The reaction system was a volume of 25.0 μL containing 12.5 μL 2 × Premix Ex TaqΙΙ (Takara, Shiga, Japan), 1.0 μL cDNA, 0.5 μM each primer (10 μM) and 10.5 μL H2O. The thermocycling parameters were one cycle at 94 °C for 3 min, 35 cycles at 94 °C for 30 s, 57 °C for 30 s and 72 °C for 30 s, and a final extension at 72 °C for 10 min. The specificity control was performed using water as template and the internal control was performed using β-actin. All PCR products were separated by 1.5% (w/v) agarose gel electrophoresis with 1 × TAE Buffer (Solarbio, Beijing, China) and observed and photographed by gel imaging and analysis system (Bio-Rad, Shanghai, China). Three technical replicates were performed.
4.4. In Situ Hybridisation of Spot/vp and Spot/vpr-Like mRNA
The fragments of Spot/vp (310bp) and Spot/vpr-like (288bp) sequences were cloned into pGEM-T easy vector (Promega, Madison, WI, USA). The linear DNAs, amplified by PCR, were used as templates for riboprobes construction using DIG-Oligonucleotide Labeling Kit (Roche Molecular Biochemicals, Mannheim, Germany). Cerebral ganglia, hepatopancreas and ovaries at early vitellogenic stage were dissected and prepared for the paraffin-cut section. The serial seven-micron sections were used for Hematoxylin-eosin (H&E) staining and in situ hybridisation [64], visualised by the BCIP/NBT Chromogen Kit (Solarbio, Beijing, China) and mounted in Clear-Mount. All sections were observed and photographed by fluorescence confocal microscope (version, Axio Imager A2) equipped with digital camera (version, AxioCam MRc) (Carl Zeiss, Jena, Germany). Three technical replicates were performed.
4.5. Temporal Expression Profiles of Spot/vp and Spot/vpr-Like mRNA
The RNAs, extracted from nervous tissues and ovary at three vitellogenic stages (n = 5 per stage), were used for cDNA synthesis. Quantitative real-time PCR (qRT-PCR) was performed by a QuantStudio™ 6 Flex Real-Time PCR (Applied Biosystems) with SYBR® Select Master Mix (TaKaRa, Shiga, Japan) according to the user manual. The internal control was performed using β-actin.
4.6. Synthetic SpOT/VP-Like Peptide Treatment In Vitro
The SpOT/VP-like peptide (CFITNCPPG-NH2) used in this study was commercially synthesised by GL Biotechnology Company Limited (Shanghai, China). The crabs at early vitellogenic stage (n = 5) were anesthetised on ice for 10 min and sterilised in 75% ethanol for 10 min. Fragments of hepatopancreas and ovaries (~0.2 g) were dissected out, washed in CPS, and precultured at 26 °C in 24-wells plates with 200 μL Leibovitz’s L-15 medium (Gibco Invitrogen Corporation, Grand Island, NY, USA) each well. One hour later, substituted the medium with L-15 medium containing different concentration of synthetic peptide (0, 10−9, 10−8, 10−7 and 10−6 M) and incubated for 6 or 12 h. Then, collected the fragments for RNA extraction and cDNA synthesis. β-actin was used as the internal control, and qRT-PCR was performed to detect the relative transcript levels of Spvg and Spvgr. Meanwhile, culture media were collected and handled according to the steroid extraction protocol, and the level of E2 in the media were measured by DetectX® SERUM 17β-ESTRADIOL Enzyme Immunoassay Kit (Arbor Assays, Ann Arbor, MI, USA). Three technical replicates were performed.
4.7. Synthetic SpOT/VP-Like Peptide Injection
The crabs at early vitellogenic stage were randomly divided into two groups (n = 5 per group), injected with 100 ng/g synthetic peptide or CPS, with the same volume, respectively. In addition, 5 crab without treatment were as initial control. Injections were given every four days for a total of 17 days duration, and on the 18th day, hepatopancreas and ovaries were collected and treated, and haemolymph was extracted and measured as above. Besides, the ovary tissues were dissected and prepared for the paraffin-cut section. The serial seven-micron sections were performed using H&E staining and the diameter of oocytes were measured. Three technical replicates were performed.
4.8. RNA Interference In Vitro
The fragments of Spot/vpr-like (478 bp) and gfp (454 bp) sequences were cloned into the pGEM-T easy vector. The linear DNAs, amplified by PCR, were used as templates for dsRNA transcribed by T7/SP6 polymerases. Hepatopancreas tissue was dissected out and treated as Section 2.7 with 200 μL L-15 media containing 5 μg Spot/vpr dsRNA or gfp dsRNA, and CPS with the same volume, respectively. After incubation at 26 °C for 10 h, substituted the media with 200 μL L-15 media containing 10−8 M synthetic peptide each well for 12 h. The hepatopancreas explants were collected for RNA extraction and cDNA synthesis. β-actin was used as internal control, and qRT-PCR was performed to detect the relative expression levels of Spot/vpr and Spvg. Three technical replicates were performed.
4.9. Statistical Analysis
The relative expression levels were calculated via the 2−ΔΔCt algorithm. All data were expressed as mean ± SD and analysed using One-way ANOVA followed by Tukey’s multiple range tests, Dunnett’ s T tests and Student’s T-tests (SPSS Statistics 18.0) to estimate the statistical differences of mean levels among the groups with statistically significant at p < 0.05 and extremely significant at p < 0.01.