Abstract
Sexual dimorphism is widespread in fish species. The red-tail catfish (Mystus wyckioides) is a commercially important catfish in the lower reaches of the Lancang River and the Mekong basin, and it shows a growth advantage in males. Here, RNA-seq was for the first time used to explore the gene expression difference between the sexes in the hypothalamus and pituitary of red-tail catfish, respectively. In the hypothalamus, 5732 and 271 unigenes have significantly higher and lower expressions, respectively, in males compared with females. KEGG analysis showed that 212 DEGs were annotated to 216 signaling pathways, and enrichment analysis suggested different levels of cAMP and glutamatergic synapse signaling between male and female hypothalami and some of the DEGs appear involved in gonad development and growth. In the pituitary, we found only 19 differentially expressed unigenes, which were annotated to 32 signaling pathways, most of which play important roles in gonad development.
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Introduction
Sexual dimorphism commonly exists in gonochoristic animals and involves many aspects of biology (Mei and Gui 2015), including body size (Ma et al. 2016; Rideout et al. 2015; Shine 1986; Wu et al. 2015), brain morphology (Gorski et al. 1978; Moriarty 1975), buccal morphology (Okuda et al. 2002), organ morphology (Adamson and King 1984; Yasuda et al. 2005), pituitary and gonadal hormones (Jalouli et al. 2003; Zimmerberg and Farley 1993), or even life expectancies (Shi et al. 2017). Fish are the most species-rich vertebrate lineage including almost half of the extant vertebrate species (Betancur-R et al. 2017). Liu first reported sex reversal phenomenon in ricefield eel (Monopterus albus), which initiated a new field on revealing the sex differentiation of fish (Bullough 1947). During the last decades, large numbers of basic studies have been reported on fish sexual dimorphism and sex determination and differentiation (Devlin and Nagahama 2002; Kobayashi et al. 2013; Scott et al. 1989; Wu et al. 2015; Li and Gui 2018a, b, Li et al. 2018).
Hypothalamus and pituitary are key endocrine glands for controlling instinctive behaviors and hormone secretion, such as metabolism, feeding, stress response, and reproduction (Dhillo et al. 2005; Harris et al. 1978; Rivier and Rivest 1991; Suchecki et al. 1993). Although the reproductive behaviors and strategies are diverse in vertebrates, the endocrine network of reproduction is conserved (hypothalamic-pituitary-gonadal axis) (Sower et al. 2009). When gonadotropin-releasing hormone (GnRH) is secreted from the hypothalamus, the gonadotropins (GTHs) are secreted in pituitary as a response. In the following, the GTHs stimulate gonads, where sex hormones are released and gonad maturation is initiated (Nozaki 2013). In addition, other adenohypophysial hormones such as growth hormone (GH), adrenocorticotropin, and prolactin are also responsive to the hypothalamic-pituitary system (Blackwell and Guillemin 1973; Heinz et al. 1995; Saga et al. 1993; Sayers et al. 1980; Salemi et al. 2007). In conclusion, hypothalamic-pituitary system is a vital element leading to physiological divergence, including sex-dependent dimorphic growth pattern (Wang et al. 2009).
Red-tail catfish (Mystus wyckioides) belongs to the catfish family Bagridae and is named after the extending filament-like ornament in its red tail. It is a native species of the Lancang River (Tippayadara et al. 2016). Interestingly, just like the other two fish in Bagridae, Pelteobagrus fulvidraco (Wang et al. 2009; Dan et al. 2013) and Pseudobagrus ussuriensis (Pan et al. 2015; Wang et al. 2009), the significant sex-dependent growth difference has been observed in red-tail catfish. However, previous studies of red-tail catfish have only focused on artificial breeding, karyotype analysis, and muscle nutrition analysis (Tippayadara et al. 2016). In the present study, we performed Illumina RNA-seq to identify differentially expressed genes and related pathways in the hypothalamic-pituitary system to reveal the molecular mechanism of sexual difference between male and female red-tail catfish. This study is the first comparative transcriptome analysis in red-tail catfish and reveals significant expression differences between males and females in hypothalamus and pituitary.
Results
Size Dimorphism Between Males and Females
Aquaculture practices and field measurement have identified the sexual dimorphism in growth. In this study, 55 4-year-old individuals (27 males and 28 females) were randomly selected, and it showed that the males had a significant growth advantage over females based on the values of body weight and body length. The average weight of females and males was 9.06 ± 2.74 kg and 11.44 ± 3.95 kg, respectively, which indicated that the weight of males was 26.27% heavier than that of females (p < 0.01) (Fig. 1a). As for the length, the average length of females and males was 93.56 ± 15.82 cm and 98.55 ± 15.83 cm, respectively, and it showed that the males were 5.33% longer than the females (p < 0.05) (Fig. 1b).
Illumina Sequencing, De Novo Assembly, and Functional Annotation
To identify differentially expressed mRNAs in hypothalamic-pituitary system between male and female red-tail catfish, two different tissues (hypothalamus and pituitary) of mature male and female adults were collected and the total RNAs from each tissue was extracted for cDNA library construction. After removing low-quality reads, a total of 47.1–48.5 (GC content = 45%, Q30 = 92.44%) and 46.6–48.3 million (GC content = 47%, Q30 = 92.51%) clean reads were obtained in the hypothalamus and pituitary, respectively (Supplementary Table 1). After trimming, these high-quality reads were de novo assembled by Trinity version20131110. Finally, a total of 89,487 unigenes with an average length of 1027.52 bp and N50 of 1792 bp were obtained in the hypothalamus, and 85,143 unigenes with average length of 1019.74 bp and N50 of 1775 bp were received in the pituitary (Supplementary Table 2). The length distributions of de novo assembled unigenes were shown in Supplementary Fig. 1.
The unigenes of two tissues were blasted against the NR, SWISSPROT, and KOG databases by using BLASTX with a threshold value of 1e−5. In NR annotation, more than half of the annotated unigenes (54.83% unigenes in the hypothalamus and 54.13% unigenes in the pituitary) were overlapped with known genes of Ictalurus punctatus (a closely related species of red-tail catfish) (Supplementary Fig. 2A and B). The numbers of annotated unigenes against databases are shown in a Wayne chart (Supplementary Fig. 2C and D). Besides that, about 60% unigenes did not match with any database entries, which may represent some non-coding RNAs or unknown protein coding genes in red-tail catfish.
Screening and Identification of Sexual Differentially Expressed Unigenes
To identify differentially expressed unigenes (DEGs) between males and females, the expression levels of assembled unigenes were determined using the reads per kilobase per million (RPKM) method. In this study, we focused on DEGs in the hypothalamus and the pituitary, respectively. Genes were considered DEGs if they showed a fold change ≥ 2 and p < 0.05 (FDR test). In the hypothalamic comparison, a total of 6003 DEGs were screened; among them, 5732 DEGs were highly expressed in males and 271 DEGs were highly expressed in females (Fig. 1c). In the pituitary, 1083 DEGs were found between genders, of which 480 were expressed significantly high in males and 603 were expressed significantly high in females (Fig. 1d). Among them, only 4 common DEGs (TAAR, Pcdh16, Gcnt3, Amhr2) were identified in both of the hypothalamus and pituitary (Supplementary Table 3).
Some important genes (GnRH, GnRHR, GHRH, etc.) involved steroid secreting in the hypothalamic-pituitary-gonadal (HPG) system, genes related to growth (IGF1/2) and aromatase secreting (CYP19A) were analyzed by performing RPKM and qRT-PCR. According to normalized value of RPKM and qRT-PCR in our studies, the greater expression of PACAP, NPY, KISS1R, IGF-1 was identified in the hypothalamus of a male, and CYP19A is highly expressed in the hypothalamus of a female (Fig. 2a). In the pituitary, FSHβ and LH are mainly expressed in female and a higher expression of PACAP was identified in male (Fig. 2b). Linear regression analysis revealed that the positive correlation between RPKM and qRT-PCR-dependent unigene expression persisted in both of the hypothalamus and pituitary with R2 = 0.86 and 0.89, respectively (Supplementary Fig. 3A and B).
GO Enrichment Analysis of DEGs
For both the hypothalamus and pituitary, DEGs were searched against the Gene Ontology database (www.geneontology.org) to infer their function according to GO annotation. In the hypothalamus, 405 DEGs were annotated to 1585 GO terms accompanied by 345 and 60 DEGs with relatively higher expression in male and female hypothalami, respectively. Ninety-eight male-highly expressed unigenes (MEGs) were annotated to nucleus (GO:0005634), 95 MEGs were annotated to cytoplasm (GO:0005737), 71 MEGs were annotated to plasma membrane (GO:0005886), 70 MEGs were annotated to DNA binding (GO:0003677), 70 MEGs were annotated to metal ion binding (GO:0046872), etc. Twenty-six female-highly expressed unigenes (FEGs) were annotated to nucleus (GO:0005634), 18 FEGs were annotated to cytoplasm (GO:0005737), 17 FEGs were annotated to ATP binding (GO:0005524), 11 FEGs were annotated to DNA binding (GO:0003677), 9 FEGs were annotated to transcription DNA-templated (GO:0006351), etc. (Fig. 3a).
In pituitary, a total of 47 DEGs were annotated into 348 GO terms. Among them, 16 male-highly expressed unigenes were related to 164 GO terms, 4 MEGs were annotated to metal ion binding (GO:0046872), 4 MEGs were annotated to plasma membrane (GO:0005886), 4 MEGs were annotated to cytoplasm (GO:0005737), 3 MEGs were annotated to extracellular space (GO:0005615), 3 MEGs were annotated to calcium ion binding (GO:0005509), etc. Thirty-one female-highly expressed unigenes were annotated to 219 GO terms. Among them, 8 FEGs were annotated to integral component of membrane (GO:0016021), 5 FEGs were annotated to extracellular exosome (GO:0070062), 5 FEGs were annotated to nucleus (GO:0005634), 4 FEGs were annotated to cytoplasm (GO:0005737), 3 FEGs were annotated to protein homodimerization activity (GO:0042803), etc.(Fig. 3b).
KEGG Enrichment Analysis of DEGs Between Males and Females
KEGG enrichment annotation can help us clarify the function of enriched DEGs in the metabolic pathways. In the hypothalamus, 212 DEGs were annotated to 216 KEGG pathways accompanied by 171 and 41 DEGs with relatively higher expression in males and females, respectively. In detail, most of the male-highly expressed unigenes (MEGs) were assigned to cAMP signaling pathway (30 MEGs, ko04024), glutamatergic synapse (30 MEGs, ko04724), circadian entrainment (29 MEGs, ko04713), calcium signaling pathway (29 MEGs, ko04020), retrograde endocannabinoid signaling (26 MEGs, ko04723), dopaminergic synapse (26 MEGs, ko04728), amphetamine addiction (24 MEGs, koko05031), insulin secretion (23 MEGs, ko04911), oxytocin signaling pathway (23 MEGs, ko04921), cGMP-PKG signaling pathway (22 MEGs, ko04022), etc. (Fig. 4a). Most of the female-highly expressed unigenes (FEGs) were assigned to cell adhesion molecules (CAMs) (4 FEGs, ko04514), aminoacyl-tRNA biosynthesis (3 FEGs, ko00970), hepatitis C (3 FEGs, ko05160), leukocyte transendothelial migration (3 FEGs, ko04670), cell cycle (3 FEGs, ko04110), viral carcinogenesis (3 FEGs, ko05203), tight junction (3 FEGs, ko04530), and axon guidance (3 FEGs, ko04360) (Fig. 4b).
The cAMP signaling pathway is involved in some fundamental functions including body growth and spermatogenesis (Skålhegg et al. 2002). Gamma-aminobutyric acid (GABA) B receptor 1 (GABBR1), adenylate cyclase 5 (ADCY5), rap guanine nucleotide exchange factor 3 (RAPGEF3), calcium/calmodulin-dependent protein kinase 2 (CAMK2), peroxisome proliferator-activated receptor alpha (PPARα), and T lymphoma invasion and metastasis-inducing protein 1 (TIAM1) were also identified as highly expressed in males (Fig. 5). Previous studies confirmed that the cAMP pathway is regulated by some glutamate receptors, which are essential in male development (Mao and Wang 2002; Winder and Conn 1993). In the glutamatergic synapse signal pathway, the glutamate receptors GRIA1, GRIA2, GRIA3, GRIA4, GRIN1, and GRIN 2B were expressed about 3.13-, 3.59-, 2.94-, 3.62-, 3.93-, and 3.16-fold higher in males compared with females (Fig. 6). Interestingly, the different expressions of CACNA1D between sexes were found in 17 KEGG pathways, ADCY5 were concentrated in 13 pathways, and PPP3C were concentrated in 9 pathways, which were enriched in most of significant KEGG pathways that may play vital role in growth sexual dimorphism or sex differentiation of red-tail catfish.
In the pituitary, only 18 DEGs were annotated to 30 pathways, 9 DEGs were highly expressed in males, and 9 DEGs were highly expressed in females. For example, the anti-Mullerian hormone type 2 receptor (AMHR2) was only identified in males and was enriched in the cytokine-cytokine receptor interaction and TGF-beta signaling pathway. While cyclin B2 (CCNB2), progesterone receptor (PGR), peroxisomal biogenesis factor 11 alpha (PAX11A), and cytochrome P450 family 26 subfamily A (CYP26A) were enriched in oocyte meiosis, p53, peroxisome, and retinol metabolism signaling pathway with higher expression in females. The desert hedgehog (DHH) was enriched in hedgehog signaling pathway and only identified in males (Table 1).
qRT-PCR Confirmation for DEGs Between Sexes
To verify accuracy of the RNA-seq data, DEGs related to mainly enriched signal pathway were randomly chosen and validated by qRT-PCR. In the hypothalamus, we analyzed fourteen DEGs, such as CACNA1D, RAPGEF3, TIAM1, PPARα, CAMK2, PPP3C, GABBR1, ADCY5, GIRIA1, GIRIA2, GIRIA3, GIRIA4, GIRIN1, and GIRIN2B, which were highly expressed in males (Fig. 7a), which was corresponded with expression data generated by qRT-PCR except CAMK2 (Fig. 7b). In the pituitary, RNA-seq showed that four genes (CYP26A, PEX11A, PGR, CCNB2) were highly expressed in the female, while DHH and Amhr2 were highly expressed in the male (Fig. 7c). Except for CCNB2, the qRT-PCR analysis confirmed the findings of the RNA-seq data (Fig. 7d). Linear regression analysis confirmed that the positive correlation between RPKM and qRT-PCR dependent unigenes expression persisted in both of the hypothalamus and pituitary with R2 = 0.87 and 0.89, respectively (Supplementary Fig. 3C and D).
Discussion
The hypothalamic-pituitary system is the most vital system for regulating reproduction and associated behaviors, and it is conserved from jawless fishes to mammals (Sower et al. 2009). The HiSeq platform has been used to compare DEGs between sexes and provide precious data for studying the sexual differentiation and its mechanism (Lin et al. 2017; Wu et al. 2015). The red-tail catfish is a native and distinctive fish in the Lancang River and also shows sexual dimorphism, such that males have a faster growth rate than females. Therefore, we performed transcriptome sequencing to identify differentially expressed genes in the hypothalamic-pituitary system between males and females in red-tail catfish.
Reproduction of animals is controlled by the hypothalamic-pituitary-gonadal (HPG) axis. In detail, if the hypothalamus is stimulated, gonadotropin-releasing hormone (GnRH) will be secreted to stimulate releasing of pituitary gonadotropins (follicle-stimulating hormone (FSH) and luteinizing hormone (LH)) (Macmanes et al. 2017; Sower et al. 2009). In this study, genes of GnRH, insulin-like growth factor I (IGF1), pituitary adenylate cyclase–activating polypeptide (PACAP), norepinephrine, neuropeptide Y (NPY), and kisspeptin (KISS1/KISS1R) were for the first time identified in the hypothalamus and pituitary of red-tail catfish. We found several key endocrine genes of GH/IGF axis highly expressed in males, coinciding with a higher level of IGF1 in male yellow catfish (Ma et al. 2016), and whose deficiency leads to dwarfism (Liu and Leroith 1999; Meyer et al. 2004; Petkovic et al. 2007). In the present work, a higher expression of KISS1R was also identified in the hypothalamus of a male, and previous studies showed that KISS1R was highly expressed in testis (Lapatto et al. 2007; Tariq et al. 2013) and brain, which was crucial for the onset of puberty in both sexes and essential for testicular function (Filby et al. 2008; Mohamed et al. 2007; Navarro et al. 2004). In our study, a higher expression of PACAP and GHRH was also identified in males, which was identical with previous findings in the half-smooth tongue sole (Ji et al. 2011). We found that LHβ and FSHβ are mainly expressed in the pituitary of females, which are the most important gonadotropins and are associated with oocyte development (Hassin et al. 1999).
It is very interesting to identify the DEGs, which are parts of specific signaling pathways that regulate sex differentiation and sexual size dimorphism. To this end, KEGG enrichment analysis was performed. In the hypothalamus, the top 20 signaling pathways were identified. The cAMP signaling pathway plays essential roles in postnatal body growth and spermatogenesis, as loss of cAMP-dependent protein kinases reduced IGF1 mRNA in the liver and would lead to defective sperm motility (Skålhegg et al. 2002; Liu and Leroith 1999). GRIAs and GRIN1 are important receptors of the glutamatergic synapse pathways. Defect of GRIAs leads to much smaller body size and reduced weight (Jia et al. 1996; Zamanillo et al. 1999). Moreover, GRIA2/4 was found to be functional in motility of spermatozoa by regulating miR-141-3p (Wu et al. 2015). Interestingly, the voltage-dependent calcium channel l type alpha-1D (CACNA1D) was confirmed to be enriched in most of KEGGs (17 of 20 KEGGs). Functional analysis found that CACNA1D-knockout mice were smaller than their littermates, as CACNA1D defect leads to significant reduction of β-cell proliferation in islets (Namkung et al. 2001). ATP2B−/− mouse also showed a lower body weight (Ver et al. 2001). ATP2B and CACNA1D are members of the histocompatibility complex I (Seuánez et al. 1997), and we suspect that CACNA1D may interact with ATP2B and regulate growth.
In the hypophysis, the cytokine-cytokine receptor interaction and oocyte meiosis pathways are indispensable during ovary development and oogenesis, because loss of function of REC8, AMHR2, and PGR leads to female infertility (Bannister et al. 2004; Hernandez Gifford et al. 2009; Lydon et al. 1995; Zhu et al. 2015). In our enriched KEGGs, PEX11A and DHH were also identified. Previous studies demonstrated that a significantly lower PEX11 may lead to higher body weight (Weng et al. 2013), and DHH appears in pre-Sertoli cells, displays male-specific transcription, and is essential for spermatogenesis (Bitgood et al. 1996).
Taken together, our study provided a new window for revealing the sexually/differently expressed genes in the hypothalamic-pituitary system. Further work will be undertaken to explore some important genes in this work to reveal sex differentiation and growth dimorphism in red-tail catfish.
Materials and Method
Sample Collection and Growth Comparison Between Males and Females
All experimental procedures of this study were permitted by the Institutional Animal Care and Institute of Hydrobiology, Chinese Academy of Sciences. The red-tail catfish involved in this study was collected in Xishuangbanna, Yunnan Province, China. Fifty-five 4-year-old individuals including 27 males and 28 females from the same parent were randomly selected. Body weight and length were compared by t test between males and females. All fish was dissected, and sex was confirmed anatomically.
Libraries Construction and Sequencing
Tissues of the hypothalamus and pituitary were sampled from 3 adult male and female individuals, respectively, and the sex was confirmed by mature testis and ovary anatomically. Total RNA was extracted by Trizol method with manufacturer’s protocol (Ambion), and Agilent 2100 Bioanalyzer (Agilent Technologies) was used to perform RNA integrity assessment. In each biological replicate, 50-μg total RNA of each tissue was used for RNA library construction. The procedures of RNA purification and synthesis of cDNA were performed by using TruSeq Stranded mRNA LTSample Prep Kit (Illumina). In detail, the mRNA was purified and concentrated by magnetic beads and then fragmented into short fragments to serve as templates for synthesizing the first strand cDNA. The double strand cDNA was synthesized and purified by agarose gel purification; after that, the cDNA fragments were coupled by sequencing adaptors at the 5′/3′ ends. The libraries of the hypothalamus and pituitary were sequenced with HiSeq 2000 platform. After wiping out the adaptor and low-quality bases, the clean paired-end reads were assembled in Trinity.pl script with the following parameters (-seqType fq -min_contig_length 200 -JM 400G -left $R1 -right $R2 -SS_lib_type RF -CPU 80) for each of tissue assemblies (Grabherr et al. 2011). The Trinity_stats.pl script was performed to obtain assembly metrics. Finally, unigenes were obtained by performing TGICL version 2.1 with default parameters (Pertea et al. 2003).
Analysis of Differentially Expressed Unigenes
To detect the differentially expressed unigenes (DEGs) between sexes in the hypothalamus and pituitary, DESeq package with the negative binomial distribution was performed to quantify the expression of two expression profiles. Fold change was performed to quantificate the differential expression and only DEGs with fold change ≥ 2, adjusted p value ≤ 0.05 (Wang et al. 2010). The false discovery rate test (adjusted p value) was applied to correct significant levels by eliminating random errors and fluctuations (Ott et al. 2012).
GO/KEGG Enrichment Analysis
The differentially expressed unigenes (DEGs) were blasted against database of NR, SWISSPROT, KOG, GO, and KEGG (p < 0.05). The statistical significance of the GO/KEGG enrichment was evaluated by the hypergeometric distribution testing, \( p=1-{\sum}_{i=0}^{m-1}\frac{\left(\begin{array}{c}M\\ {}i\end{array}\right)\left(\begin{array}{c}N-M\\ {}n-i\end{array}\right)}{\left(\begin{array}{c}N\\ {}n\end{array}\right)} \), in which N represents the number of unigenes with GO/KEGG annotation, n represents number of DEGs with GO/KEGG annotation, M represents number of unigenes with one specific GO/KEGG annotation, and m represents the number of DEGs with one specific functional annotation (Hassin et al. 1999). A smaller p value presented a more abundant enrichment.
Quantitative Real-Time PCR
For verifying the results of analysis of DEGs, total RNA of the hypothalamus and pituitary from both sexes was reverse-transcribed by using the PrimeScriptRT reagent Kit (Takara) following the manufacturer’s protocol. The quantitative real-time PCR (qRT-PCR) reaction was performed using a Roche LightCycler 480 instrument with SYBR Green PCR master mix (Roche). Five biological replicates were performed in each reaction. The expression of β-actin was used as reference to normalize the Ct values to conduct the 2−ΔΔCt method (Nolan et al. 2006). The differential expression analysis was confirmed by ANOVA analysis (Anderson 2010). The sequences of primers involved in this study were Supplementary Table 4.
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Funding
This work was supported by National Key R&D Program of China (2018YFD0901201), the Key Program of Frontier Sciences of the Chinese Academy of Sciences (QYZDY-SSW-SMC025), the Yunnan Academician Workstation (Y73Z04-1-301), the earmarked fund for Modern Agro-industry Technology Research System (NYCYTX-49), and the Autonomous Project of the State Key Laboratory of Freshwater Ecology and Biotechnology (2016FBZ01).
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All experiments and animal treatments were approved by the Institute of Hydrobiology Institutional Animal Care and Use Committee (approval ID, keshuizhuan 0829).
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Supplementary Fig. 1
Length distribution of the de novo assembled unignes. (PNG 487 kb)
High resolution image
(TIF 2665 kb)
Supplementary Fig. 2
Stastics of species distribution of Blast hits and annotated unigenes against NR, KOG, GO, KEGG and SWISSPROT database. (A), Stastics of annotated unigenes in hypothalamus. (B), Stastics of annotated unigenes in pituitary. (C), Species distribution of hypothalamic Blast hits against NR database. (D), Species distribution of pituitary Blast hits against NR database. (PNG 2711 kb)
High resolution image
(TIF 62438 kb)
Supplementary Fig. 3
Linear regression analysis of expression data generated by RNA-seq and qRT-PCR. X-axis represents log2(mean normalized RPKM), Y-axis represents log2(mean normalized qRT-PCR). (PNG 212 kb)
High resolution image
(TIF 8647 kb)
Supplementary Table 1
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Supplementary Table 2
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Supplementary Table 3
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Supplementary Table 4
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Wu, JJ., Zhou, YL., Wang, ZW. et al. Comparative Transcriptome Analysis Reveals Differentially Expressed Genes and Signaling Pathways Between Male and Female Red-Tail Catfish (Mystus wyckioides). Mar Biotechnol 21, 463–474 (2019). https://doi.org/10.1007/s10126-019-09894-x
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DOI: https://doi.org/10.1007/s10126-019-09894-x