Abstract
MicroRNAs (miRNAs), a group of small molecule non-encoding RNAs, are key post-transcriptional regulators of gene expression that are implicated in many biological processes. In the current study, miR-217 from Eriocheir sinensis was selected for studying its roles during host–virus interaction. Overexpression or silencing of miR-217 led to considerable effects on white spot syndrome virus (WSSV) replication, implying that miR-217 played a positive role in WSSV infection. In insect High Five cells, miR-217 significantly inhibited Tube gene expression by binding to the 3′-untranslated region of the Tube. Overexpression of miR-217 in crab led to downregulation of tube expression. Knockdown of Tube in vivo led to significant enhancement of WSSV infection and inhibited the expression of five antimicrobial peptide (AMP) genes (Anti-lipopolysaccharide factor ALF1, ALF2, ALF3; Crustin Crus1, Crus2) in WSSV-challenged crabs. Overexpression of miR-217 also led to downregulation of these AMP genes in WSSV-challenged crabs. Our results showed that host miRNA played positive roles in virus infection by regulation of host tube gene, which is the key component of Toll signaling pathway.
Introduction
MicroRNAs (miRNAs) are a class of small non-coding RNAs that are found in diverse eukaryotic organisms (Carrington and Ambros, 2003). MicroRNAs are endogenous, 18 to 26 nucleotides (nt) long, and are processed from the hairpin transcripts cleaved by two RNase III enzymes, namely, Drosha and Dicer (Bernstein et al., 2001; Bartel, 2004). The mature miRNA strand is incorporated into the RNA-induced silencing complex, wherein mRNA degradation or protein translation repression is controlled mainly through acting on the 3′-untranslated region (UTR) of target mRNAs (Schwarz et al., 2003; Meister and Tuschl, 2004; Bagga et al., 2005). Since lin-4 and let-7, the first miRNAs, were discovered in Caenorhabditis elegans (Lee et al., 1993; Reinhart et al., 2000), numerous miRNAs have been found to be involved in the regulation of diverse biological processes, including development, differentiation, apoptosis, oncogenesis, and immune activation (Ambros, 2004; Lecellier et al., 2005; Pedersen et al., 2007). Host miRNAs are believed to be key regulators of virus–host interactions (Triboulet et al., 2007; Umbach and Cullen, 2009). For example, human miR-125a has been shown to suppress the replication of hepatitis B virus by binding the viral transcript encoding the surface antigen and interfering with its expression (Mosca et al., 2014). MiR-155 inhibits Japanese encephalitis virus replication and negatively modulates innate immune responses in JEV-infected human microglial cells (Pareek et al., 2014). Two host cellular miRNAs, namely, miR-320a and miR-140, were found to inhibit mink enteritis virus infection into feline kidney cells by repression of its receptor, feline transferrin receptor (Sun et al., 2014). Host miR-26a suppresses the replication of porcine reproductive and respiratory syndrome virus by upregulating the expression of type I interferon, as well as the IFN-stimulated genes MX1 and ISG15 (Li L. et al., 2015). However, a small amount of information is available regarding the pathways mediated by host miRNAs in invertebrates.
Invertebrates lack antibodies and complements; however, they can initiate a rapid and effective innate immune response against pathogenic organisms (Uematsu and Akira, 2008). Recognizing invading microbial pathogen, which is conducted by a set of so-called pattern recognition receptors (PRRs), is an essential step in innate immune responses (Bischoff et al., 2004). Toll-like receptors or Tolls, which initiate innate immune responses by sensing pathogen-associated molecular patterns (Kawai and Akira, 2010) and then activating evolutionarily conserved Toll signal transduction (Imler and Hoffmann, 2001), are the most extensively studied PRRs. Toll signaling occurs through several adaptor proteins, such as myeloid differentiation factor 88 (MyD88), Tube, and Pelle (Valanne et al., 2011). Upon ligand binding, MyD88 recruits the activated Toll receptor and the cytosolic adaptor Tube to transfer Toll signaling. Then, Pelle is recruited to the vicinity of Tube, forming a trimeric complex (MyD88-Tube-Pelle) mediated by the death domain of Tube. Finally, the signal is transmitted to the Dorsal/Cactus complex that regulates the Toll-dependent gene expression, such as antimicrobial peptides (AMPs), as well as a substantial number of other innate immune responsive genes (Belvin and Anderson, 1996; Lemaitre and Hoffmann, 2007; Valanne et al., 2011). The adaptor Tube is an essential component of the Toll signaling pathway. The Drosophila melanogaster Tube not only participates in dorsoventral axis formation during development but is also involved in regulating diverse downstream signaling as well as the response against gram-positive bacteria and fungi (Lemaitre et al., 1996; Wang et al., 2006). The mud crab Scylla paramamosain, SpTube, together with SpPelle and SpMyD88, may form a trimeric complex in the Toll signaling cascade and are shown to be involved in the immunity against gram-positive and gram-negative bacteria (Li et al., 2013). EsTube might play important roles in the innate immune response to exogenous pathogenic stimulation and the development of the gonads in the Chinese mitten crab, Eriocheir sinensis (Yu et al., 2014). Therefore, Tube may have a vital role in initiating and activating the immune system. However, the host–virus interaction between Tube and miRNAs is not addressed at present.
White spot syndrome virus (WSSV) is one of the most virulent agents threatening the shrimp culture industry worldwide (Escobedo-Bonilla et al., 2008). Recently, one report showed that WSSV also caused serious disease, thereby threatening the Chinese mitten crab aquaculture industry (Ding et al., 2015). Given the breadth of miRNA-mediated regulation of immunity, the role of host miRNAs in WSSV infection is of significant interest. Herein, the crab miR-217 targeting Tube was characterized in this study. Our findings indicated that miR-217 first directly targeted Tube. Then, it regulated the expression of AMP genes. Finally, miR-217 promoted the WSSV infection in E. sinensis.
Materials and methods
Crab culture and WSSV challenge
Approximately 40 g of E. sinensis was raised in a group of 30 individuals at room temperature. Three crabs from each group were randomly selected for the PCR detection of WSSV with WSSV-specific primers (5′-TATTGTCTCTCCTGACGTAC-3′ and 5′-CACATTCTTCACGAGTCTAC-3′) to ensure that the crabs were virus-free before experiments. Then, the virus-free crab was infected with 100 μl WSSV solution for each crab at 105 copies/ml by intramuscular injection. At different times post-infection (0, 2, 4, 6, 12, 24, 36, 48, 60, and 72 h), the hemolymph was collected from treated crabs and subsequently centrifuged at 2000 rpm at 4°C for 10 min to harvest the hemocytes. Other tissues (heart, hepatopancreas, gills, muscles, intestines, nerves, and eyestalk) from the five untreated crabs were also collected for later use.
Detection of crab miR-217 using real-time PCR
Total RNAs were extracted from the preceding issues mentioned using the mirVana miRNA isolation kit following the instructions of the manufacturer (Ambion, USA). cDNA for miRNA qRT-PCR was then synthesized with All-in-one™ miRNA First-Strand cDNA Synthesis Kit (GeneCopoeia™, USA) according to the protocol of the manufacturer. Quantitative real-time PCR was carried out according to the protocol of All-in-one™ miRNA qRT-PCR Detection Kit (GeneCopoeia™, USA) using the miR-217 special primer (5′-CGCTACTGCATCAGGAACTGA-3′). Glyceraldehyde-3-phosphate dehydrogenase (GAPDH) was used as a control. The first-strand cDNA synthesis was obtained by using the PrimeScript™ RT reagent Kit (Perfect Real Time) (Takara, Dalian, China), and qRT-PCR was carried out using 2 × SYBR Premix Ex Taq kit (Takara, Japan) with GAPDH-specific primers (5′-CTGCCCAAAACATCATCCCATC-3′ and 5′-CTCTCATCCCCAGTGAAATCGC-3′).
Silencing or overexpression of miR-217 in crab
The anti-miRNA-217 oligonucleotide (AMO-miR-217: 5′-ATCCAATCAGTTCCTGATGCAGTA-3′, 10 nM) and WSSV (105 copies/ml) were coinjected into crab to silence the expression of miR-217. As a control, the sequence of AMO-miR-217 was scrambled, yielding AMO-miR-217-scrambled (5′-CACTAAGTGGATGCTAAACTTCTC-3′). The AMO-miR-217-scrambled (10 nM) and WSSV (105 copies/ml) were included in the injections. The oligonucleotides were sequentially injected into the same crab twice at a 16 h interval to avoid the degradation of AMO-miR-217 or AMO-miR-217-scrambled in crab. WSSV alone (105 copies/ml) and phosphate buffer saline (PBS) were also injected into crab. At 24, 36, and 48 h after the last injection, the hemolymph specimens selected at random from three crabs were mixed and subjected to subsequent analysis.
The mimic of miR-217 (5′-UACUGCAUCAGGAACUGAUUGGAU-3′) was synthesized with an in vitro transcription T7 kit for siRNA synthesis (Takara, Japan). The sequence of miR-217 was scrambled to generate the control miR-217-scrambled (5′-CUCAAGGAUGCGUUAAGGUUACUA-3′). miRNA (20 μg) and WSSV (105 copies/ml) were coinjected into healthy crabs to overexpress miR-217. At 16 h after the coinjection, the miRNA (20 μg) (100 μl /crab) was injected into the same crab. As controls, miR-217-scrambled, WSSV (105 copies/ml), and PBS were included in the injections. At different time points after the last injection, the hemolymph specimens from three crabs were selected. All the preceding assays described were biologically repeated for three times.
Quantitative analysis of WSSV copies by real-time PCR
The genomic DNA was extracted to quantify the WSSV copies in crab. qRT-PCR was performed with WSSV-specific primers (5′-TTGGTTTCATGCCCGAGATT-3′ and 5′-CCTTGGTCAGCCCCTTGA-3′) and a TaqMan probe (5′-FAM-TGCTGCCGTCTCCAA-TAMRA-3′). The plasmid containing a DNA fragment of 1,400 bp from the WSSV genome was used as the internal standard of real-time PCR (Liu et al., 2009). The 25 μl PCR reaction solutions contained 12.5 μl of the Premix ExTaq (Takara, Japan), 0.5 μl of 10 μM primers each, 1 μl of 10 μM TaqMan fluorogenic probe, 1 μl of DNA template, and 9.5 μl of distilled water. The pre-denaturalization stage of the PCR program was 95°C for 1 min, followed by the amplification stage comprising 40 cycles of 95°C for 30 s, 52°C of 30 s, and 72°C for 30 s.
Prediction and identification of target genes of miR-217 in crab
Owing to the insufficient crab genome sequence, the assembled crab EST sequences (unpublished) were used to predict the target genes of miR-217 in crab. Three computational algorithms, including TargetScan 5.1 (http://www.targetscan.org), miRanda (http://www.microrna.org/), and Pictar (http://pictar.mdc-berlin.de/), were conducted. The data predicted by the three algorithms were overlapped and calculated.
Plasmid constructions
To explore the interaction between miR-217 and its target gene Tube, the enhanced green fluorescent protein (EGFP) gene was amplified from the pEGFP vector (BD Biosciences, USA) using EGFP forward and reverse primers (5′-AAGAGCTCGGATCCCCGGGTAC-3′ and 5′-AATCTAGAGTCGCGGCCGCTTTA-3′) and cloned into the pIZ/V5-His vector (Invitrogen, USA) to produce a control EGFP construct. Subsequently, the Tube 3′UTR was cloned downstream of the EGFP gene using the XbaI and SacII restriction sites. The primers used for the amplification of Tube 3′UTR were 5′-GCTCTAGATGATGGCTGCATTCACTTGG-3′ and 5′-TCCCCGCGGTAATTACATTGATGATATCA-3′. The sequence of Tube 3′UTR complementary to the miR-217 seed sequence (ATGCAGT) was randomly mutated to CGTACTG, generating the EGFP-ΔTube construct. The amplification of ΔTube 3′UTR was conducted by PCR with sequence-specific primers 5′-GGATAGAAAATGTGTCCACGTACTGACCTCATGG-3′ and 5′-ATCTTCTTACCATGAGGTCAGTACGTGGACACATT-3′. Recombinant plasmids were confirmed by sequencing.
Cell culture, transfection, and fluorescence assays
Insect High Five cells (Invitrogen) were cultured at 28°C in Express Five serum-free medium (SFM, Invitrogen) containing L-glutamine (Invitrogen). The cells were cotransfected with the EGFP, EGFP-Tube, or EGFP-ΔTube plasmid and the synthesized miR-217 (miR-217-mimic) using the Cellfectin transfection reagent (Invitrogen) according to the protocol of the manufacturer. The concentrations of miR-217-mimic and the plasmid were 200 nM/well and 400 ng/well, respectively. As a control, the control miRNA was included in the cotransfection. All the miRNAs were synthesized by Shanghai GenePharma Co., Ltd. (Shanghai, China). At 48 h after cotransfection, the EGFP fluorescence of the cells was measured by a Flex Station II microplate reader (Molecular Devices, USA) at 490/510 nm of excitation/emission (Ex/Em).
RNAi assays in crab in vivo
Based on the sequences of crab Tube gene, siRNA (Tube-siRNA: 5′-CCCAAACGGCAACCCUCAU-3′) was synthesized according to the design rule for siRNA. The sequence of siRNA was randomly scrambled to generate the control siRNA, Tube-siRNA-scrambled (5′-UCACCUACGCACCACACAG-3′). To silence Tube expression, Tube-siRNA (20 μg) and WSSV (105 copies/ml) were coinjected into each crab. Sixteen hours later, the siRNA was injected into the same crab at 20 μg/crab. WSSV (105 virus copies/ml) alone was used as a positive control. At different times (24, 36, and 48 h) after the injection of siRNA, the crab hemocytes was collected and stored at −80°C for later use.
Quantification of mRNA with real-time PCR
The mRNA levels of Tube and AMP genes in crab were determined using qRT-PCR. The Tube primers were 5′-ATTGTGCTGCTGGAGTTGCTGAC-3′ and 5′-CATCGTCGGTCGCTTCTTCTTGG-3′. Anti-lipopolysaccharide factor 1 (ALF1), ALF2, ALF3, Crustin 1 (Cru1), and Crustin 2 (Cru2) were detected with sequence-specific primers (ALF1-RT-F: 5′-GACGCAGGAGGATGCTAAC-3′, and ALF1-RT-R: 5′-TGATGGCAGATGAAGGACAC; ALF2-RT-F: 5′-GACCCTTTGCTGAATGCTTGA-3′, and ALF2-RT-R: 5′-CTGCTCTACAATGTCGCCTGA-3′; ALF3-RT-F: 5′-ACGAGGAGCAAGGAAAGAAAG-3′, and ALF3-RT-R: 5′-TTGTGCCATAGACCAGAGACTT-3′; Crus1-RT-F: 5′-GCTCTATGGCGGAGGATGTCA-3′, and Crus1-RT-R: 5′-CGGGCTTCAGACCCACTTTAC-3′; Crus2-RT-F: 5′-GCCCACCTCCCAAACCTAT-3′, and Crus2-RT-R: 5′-GCAAGCGTCACAGCAGCACT-3′). Crab GAPDH was used as the internal reference. The 2−ΔΔCT method was used to calculate the relative fold-change of the mRNA expression level (Livak and Schmittgen, 2001).
Statistical analysis
Numerical data were analyzed using one-way analysis of variance to calculate the mean and standard deviation of triplicate assays. Unpaired sample t-test was conducted, and the differences were considered significant if P < 0.05 or P < 0.01.
Results
Effects of miR-217 on virus infection in crab
MiR-217 expression in several tissues was performed by qRT-PCR (Figure 1A). GAPDH was used as a reference. MiR-217 was mainly expressed in gills and hemocytes, with a relatively low expression level in the hepatopancreas, intestine, and muscle. The expression changes of miR-217 in WSSV-challenged crab were detected to explore the relationship between miR-217 and WSSV infection. From the result of qRT-PCR, the WSSV infection led to a significant increase of miR-217 expression level in the hemocytes of crab (Figure 1B). MiR-217-silenced or overexpressed crabs were analyzed with the assays of the WSSV copies to further evaluate the role of miR-217 in the virus infection. The data presented that the WSSV copies were significantly increased by the miR-217 overexpression and significantly decreased by the miR-217 silencing compared with the control (Figures 1C,D), indicating that miR-217 played a positive role in regulation of the WSSV infection.
Figure 1
Interaction between host miR-217 and host Tube gene in vitro
Growing evidence has indicated that host miRNAs play important roles in host–virus interactions in invertebrates. In this study, the prediction results indicated that the crab miR-217 could target the host Tube (GenBank Accession No. KC011815), an important adaptor protein of the Toll pathway (Figure 2A). MiR-217-mimic and the plasmid EGFP-Tube were cotransfected into High Five cells because a crab cell line was unavailable (Figure 2B) to evaluate the direct interaction between miR-217 and Tube. The results revealed that the fluorescence intensity in the cotransfected cells was significantly weaker than that in the controls, showing that miR-217 targeted the Tube gene (Figures 2C,D). EGFP-ΔTube was constructed to investigate the specificity of the interaction between miR-217 and Tube 3′UTR. The result showed that miR-217-mimic had no effect on the expression of EGFP in miR-217-mimic and EGFP-ΔTube cotransfected cells, showing that miR-217 seed sequence was required to target the Tube 3′UTR.
Figure 2
Interaction between miR-217 and Tube gene in vivo
MiR-217-mimic was injected into WSSV-infected crab to reveal the in vivo interaction between miR-217 and Tube gene in crab. The results indicated that overexpression of miR-217 led to a significant decrease in the transcript levels of the Tube gene at 24, 36, and 48 h post-infection (Figure 3A). AMO-miR-217 was injected into WSSV-infected crab to inhibit the expression of endogenous miR-217. The results showed that crab Tube expression was enhanced by AMO-miR-217 (Figure 3B). These results showed that changes in miR-217 levels could alter the expression of the host gene Tube in crab in vivo.
Figure 3
Roles of Tube in crab–virus interaction
QRT-PCR was used to analyze the Tube mRNA level after WSSV infection. At 24, 36, 48, 60, and 72 h in response to WSSV infection, the crab Tube was significantly upregulated (Figure 4A). The expression of the crab Tube gene was silenced by sequence-specific siRNA, followed by the examination of WSSV copies to further examine the roles of Tube in virus infection. The qRT-PCR result showed that the expression of Tube was repressed by the gene-specific siRNA from 24 h to 48 h after siRNA injection (Figure 4B). The mutation-siRNA had no effect on the expression of Tube. The data indicated that the Tube-siRNA was highly sequence specific, which could silence the Tube gene in crab in vivo. When the Tube gene had been silenced by Tube-siRNA, the numbers of WSSV genome copies/mg in crab hemocytes significantly increased compared with the control (WSSV only and Tube-siRNA-scrambled) (Figure 4C). The data indicated that Tube gene played important roles in WSSV replication.
Figure 4
AMP genes expression are regulated by Tube
AMP genes are important effectors of the Toll pathway in invertebrates. The expression of Tube was knocked down in crab to reveal the relationship between Tube and AMP genes ALF1 (Accession No. DQ793214), ALF2 (GU014699), ALF3 (HQ850572.1), Crus1 (GQ200832), and Crus2 (GQ200833). Under the conditions wherein the Tube gene expression was silenced, five AMP gene expression levels were detected by qRT-PCR. The results are shown in Figure 5, wherein the mRNA transcriptions of AMPs were increased by different degrees of magnitude after the WSSV challenge. However, the expression levels of these AMPs were significantly decreased in the Tube-siRNA experimental group compared with the controls (Tube-siRNA-scrambled, WSSV only). Therefore, ALF1, ALF2, ALF3, Crus1, and Crus2 are possibly the downstream genes of Tube.
Figure 5
AMP genes expression are regulated by miR-217
All the preceding results described implied that five AMP genes are the downstream effector genes regulated by Tube. Therefore, the pathway mediated by host miR-217 was further explored. The results indicated that the expression levels of ALF1 (Figure 6A), ALF2 (Figure 6B), ALF3 (Figure 6C), Crus1 (Figure 6D), and Crus2 (Figure 6E) are significantly downregulated when miR-217 is overexpressed in crab. By contrast, the control miRNA injection had no effect on the transcription of these AMP genes. The knockdown of miR-217 by AMO-miR-217 led to a significant increase in the expression levels of ALF1 (Figure 7A), ALF2 (Figure 7B), ALF3 (Figure 7C), Crus1 (Figure 7D), and Crus2 (Figure 7E) at 24 h to 48 h post-infection compared with those of WSSV only. By contrast, the control AMO-miR-217-scrambled had no effect on the transcriptions of AMPs, thereby suggesting that the host miR-217, ALF1, ALF2, ALF3, Crus1, and Crus2 shared the same pathway.
Figure 6
Figure 7
Expression of ALF1, ALF2, ALF3, Crus1, and Crus2 during virus infection in crab
The genes of ALF1, ALF2, ALF3, Crus1, and Crus2 were characterized and their expression patterns were performed in crabs to evaluate their roles in viral infection. As shown in Figures 8A–E, the mRNAs of ALF1, ALF2, ALF3, Crus1, and Crus2 were upregulated post-WSSV infection at several time points. By contrast, the transcripts of the five AMP genes did not obviously change after PBS challenge. The data demonstrated that the five AMP genes might be involved in anti-viral innate immune defense. These findings together revealed that host miRNA (miR-217) inhibited the Toll signaling pathway by targeting the host Tube gene, resulting in the enhancement of virus replication in crabs (Figure 8F).
Figure 8
Discussion
Although Toll signaling pathway has been implicated in the processes of virus infection, its function in host–virus interaction remains to be unfamiliar. MiRNAs are post-transcriptional regulatory molecules that could regulate gene expression and participate in numerous key biological processes by inhibiting mRNA translation or promoting mRNA decomposition (Meister and Tuschl, 2004; Bagga et al., 2005). Tumor-secreted miRNAs (miR-21 and miR-29a) can function as ligands, binding to the receptors of the Toll-like receptor (TLR) family, namely, murine TLR7 and human TLR8 (Fabbri et al., 2012). Human miR-9 was rapidly increased after TLR4-activation, which operated a feedback control of the NF-κB-dependent responses by fine-tuning the expression of a key member of the NF-κB family (Bazzoni et al., 2009). MiR-105 was reported as a modulator of TLR2 translation in human gingival keratinocytes (Benakanakere et al., 2009). MiR-146 could control TLR and cytokine signaling through a negative feedback regulation loop involving the downregulation of IL-1 receptor-associated kinase 1 and TNF receptor-associated factor 6 protein levels (Taganov et al., 2006). However, miRNAs of crustaceans that mediate the regulation of key components of the host Toll pathway are still not well studied.
In the current study, we reported that crab-specific miR-217 played positive roles in WSSV infection by negatively regulating host Toll signaling pathway in E. sinensis. MiR-217 inhibited the Toll signaling pathway by targeting the Tube gene. Tube, which is the key component of host Toll pathway, played pivotal roles in numerous biological activities, such as survival, development, and innate immunity (Yu et al., 2014). The Tube could activate or repress a broad range of downstream genes and be involved in forming a sophisticated network in response to various stress signals. In many cases, an individual miRNA can target a unique gene and lead to subsequent changes of the biological processes associated with this target gene. The overexpression of crab miR-217 through the injection of miR-217-mimic led to the enhancement of WSSV copies, implying that miR-217 plays a positive role in WSSV replication. In the multinuclear-activation of galactosidase indicator cells, human miR-217 could influence the transactivation of Tat-induced human immunodeficiency virus 1 through the downregulation of SIRT1 expression (Zhang et al., 2012). In crustaceans, host miRNAs were also found to be involved in virus infection. In Marsupenaeus japonicas, host miR-1000 was reported to contribute considerable effects on apoptosis and WSSV replication through targeting p53 (Gong et al., 2015). Shrimp miR-7 could serve as an antiviral factor by interacting with viral wsv477 (Huang and Zhang, 2012). In Macrobrachium rosenbergii, host miR-9041 and miR-9850 played positive roles in WSSV replication by targeting the STAT gene (Huang Y. et al., 2016). Our investigations revealed that crab miR-217 led to a decrease in the transcript level of the Tube gene, resulting in the enhancement of WSSV copies.
AMP genes are effector molecules in the innate immunity of invertebrates (Hancock et al., 2006). The AMPs of major crustaceans are represented by three cationic peptide families: ALFs, crustins, and penaeidins (Tassanakajon et al., 2010). ALFs are cationic AMPs with the ability to bind and neutralize lipopolysaccharide and are crucial bioactive substances in the innate immunity of crustaceans (Aketagawa et al., 1986). Crustins are cationic cysteine-rich AMPs (Liu et al., 2015). In E. sinensis, three ALF genes (ALF1, ALF2, and ALF3) and two Crustin genes (Crus1 and Crus2) were identified. The upregulated expression of the five AMP genes in WSSV-challenged crabs may indicate their possible roles in anti-virus immune defense. ALF from Fenneropeneaus chinensis played a key role in inhibiting WSSV replication (Li S. et al., 2015). In Penaeus monodon, the enhanced crustin-like AMP conferred significant protection from WSSV infection (Antony et al., 2011). The knockdown of Tube gene resulted in a reduction of ALF1, ALF2, ALF3, Crus1, and Crus2 transcripts in crabs. These results suggested that crab AMP genes could be modulated by the host Toll pathway, which is also the case in Drosophila (Lemaitre and Hoffmann, 2007). Similarly, in Procambarus clarkii, PcToll was involved in the regulation of Crus expression (Wang et al., 2015). The knockdown of Dorsal in M. rosenbergii resulted in the suppression of Crus transcripts (Huang X. et al., 2016). The silencing of the PmMyD88 gene resulted in a decrease of expression of two Crus genes in Litopenaeus vannamei (Arayamethakorn et al., 2017). Therefore, we identified several AMP genes regulated by crab tube in our study. Further experiments indicated that overexpression of miR-217 inhibited the expression of these AMP genes. Hence, our findings together revealed that host miRNA (miR-217) targeting the host tube gene caused the inhibition of the expression of AMP genes, resulting in the enhancement of virus replication in crabs.
Funding
The current study was supported by the National Natural Science Foundation of China (Grant Nos. 31572647, 31272686), Natural Science Fund of Colleges and universities in Jiangsu Province (14KJA240002), High level talents in Nanjing Normal University Foundation (2012104XGQ0101), Graduate students Research and Innovation Program of Jiangsu Province (KYZZ15_0214), Jiangsu Agriculture Science and Technology Innovation Fund (CX(15)1011-02) and the Project Funded by the Priority Academic Program Development of Jiangsu Higher Education Institutions (PAPD).
Conflict of interest statement
The authors declare that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest.
Statements
Author contributions
YH, KH, and QR carried out the experiments. YH, WW, and QR designed the experiments and analyzed the data. YH and QR contributed reagents/materials. YH and QR wrote the manuscript. All authors gave final approval for publication.
Conflict of interest
The authors declare that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest.
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Summary
Keywords
Eriocheir sinensis, WSSV, miR-217, toll signaling pathway, Tube, antimicrobial peptides
Citation
Huang Y, Han K, Wang W and Ren Q (2017) Host MicroRNA-217 Promotes White Spot Syndrome Virus Infection by Targeting Tube in the Chinese Mitten Crab (Eriocheir sinensis). Front. Cell. Infect. Microbiol. 7:164. doi: 10.3389/fcimb.2017.00164
Received
31 January 2017
Accepted
18 April 2017
Published
04 May 2017
Volume
7 - 2017
Edited by
Dongsheng Zhou, Beijing Institute of Microbiology and Epidemiology, China
Reviewed by
Rosalba Giugno, University of Verona, Italy; César López-Camarillo, Universidad Autónoma de la Ciudad de México, Mexico
Updates
Copyright
© 2017 Huang, Han, Wang and Ren.
This is an open-access article distributed under the terms of the Creative Commons Attribution License (CC BY). The use, distribution or reproduction in other forums is permitted, provided the original author(s) or licensor are credited and that the original publication in this journal is cited, in accordance with accepted academic practice. No use, distribution or reproduction is permitted which does not comply with these terms.
*Correspondence: Wen Wang njnuwang@263.net
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