Analysis of Expression, Cellular Localization, and Function of Three Inhibitors of Apoptosis (IAPs) from Litopenaeus vannamei during WSSV Infection and in Regulation of Antimicrobial Peptide Genes (AMPs)

Inhibitors of apoptosis (IAPs) play important roles in apoptosis and NF-κB activation. In this study, we cloned and characterized three IAPs (LvIAP1-3) from the Pacific white shrimp, Litopenaeusvannamei . LvIAP1-3 proteins shared signature domains and exhibited significant similarities with other IAP family proteins. The tissue distributions of LvIAP1-3 were studied. The expression of LvIAP1-3 was induced in the muscle after white spot syndrome virus (WSSV) infection. LvIAP1 expression in the gill, hemocytes, hepatopancreas, and intestine was responsive to WSSV and Vibrio alginolyticus infections. LvIAP2 expression in the gill, hemocytes, and hepatopancreas was also responsive to WSSV infection. The expression of LvIAP3 in the gill, hemocytes, and intestine was reduced after V . alginolyticus infection. When overexpressed in Drosophila S2 cells, GFP labeled-LvIAP2 was distributed in the cytoplasm and appeared as speck-like aggregates in the nucleus. Both LvIAP1 and LvIAP3 were widely distributed throughout the cytoplasm and nucleus. The expression of LvIAP1, LvIAP2, and LvIAP3 was significantly knocked down by dsRNA-mediated gene silencing. In the gill of LvIAP1- or LvIAP3-silenced shrimp, the expression of WSSV VP28 was significantly higher than that of the dsGFP control group, suggesting that LvIAP1 and LvIAP3 may play protective roles in host defense against WSSV infection. Intriguingly, the LvIAP2-silenced shrimp all died within 48 hours after dsLvIAP2 injection. In the hemocytes of LvIAP2-silenced shrimps, the expression of antimicrobial peptide genes (AMPs), including Penaeidins, lysozyme, crustins, Vibrio penaeicidae-induced cysteine and proline-rich peptides (VICPs), was significantly downregulated, while the expression of anti-lipopolysaccharide factors (ALFs) was upregulated. Moreover, LvIAP2 activated the promoters of the NF-κB pathway-controlled AMPs, such as shrimp Penaeidins and Drosophila drosomycin and attacin A, in Drosophila S2 cells. Taken together, these results reveal that LvIAP1 and LvIAP3 might participate in the host defense against WSSV infection, and LvIAP2 might be involved in the regulation of shrimp AMPs.


Introduction
Apoptosis is a genetically programmed process of controlled cell suicide that plays critical roles in organismal development, homeostasis, and the immune system through elimination of cells that are no longer useful [1]. The dysregulation of apoptosis contributes to the pathogenesis of various diseases, such as cancers and autoimmunity [2,3]. Because of its destructive effect on living cells, apoptosis is tightly controlled by multiple regulators [4]. Inhibitors of apoptosis proteins (IAPs) inhibit the activity of caspases, the main executors of the apoptosis process, and play important roles in regulating the progression of apoptosis from insects to humans [4,5]. IAP was first identified as a baculovirus gene that inhibits apoptosis in virus-infected Spodoptera frugiperda insect cells to enhance viral multiplication [5]. Since then, many IAP homologs have been identified in yeast, nematodes, flies, and mammals [5]. There are four and eight members of the IAP family in Drosophila and humans, respectively [5]. The IAP family proteins are characterized by the presence of one to three Nterminal zinc-binding baculoviral IAP repeat (BIR) domains [6]. These BIR domains bind directly to the caspases and inhibit their activities. Therefore, BIR domains are essential for the anti-apoptotic properties of IAPs [6]. Some IAPs also contain a C-terminal RING domain, which has ubiquitin E3 ligase activity [6]. The RING domain ubiquitinates the proteins that bind to IAPs, including caspases and IAPs themselves [6]. The ubiquitinated caspases are inactivated and the ubiquitinated IAPs are subjected to proteasome degradation [6].
In addition, IAPs also play important roles in immune signaling regulation from insects to mammals [6][7][8]. In Drosophila, the Toll and immune deficiency (IMD) pathways are the major regulators of the immune responses [9][10][11]. Gram-positive bacteria and fungi activate the Toll pathway, while Gram-negative bacterial infections activate the IMD pathway [9][10][11]. Activation of the Toll and IMD pathways initiates an intracellular signaling cascade to activate the NF-κB family proteins Dorsal/Dif and Relish, respectively, promoting the expression of immune-related genes, such as antimicrobial peptide genes (AMPs) [9][10][11]. Although no components of Drosophila Toll and IMD pathways have been identified as detectors for viral infections, viruses activate both pathways, which contribute to the restriction of viral replication [12][13][14]. Knock-down of Drosophila IAP2 (DIAP2) in insect cells reduced the expression of AMPs induced by Gram-negative bacteria, suggesting a role of DIAP2 in the IMD pathway [15][16][17][18]. The RNAi-mediated silencing of DIAP2 in the adult fat body also abrogated AMP gene expression induced by Gram-negative bacterial infection. Importantly, DIAP2 null flies exposed to Gram-negative bacteria did not activate the IMD pathway and died [15][16][17][18]. The exogenous expression of wild-type DIAP2, but not the E3-deficient RING mutant, rescued the DIAP2 null flies [16,18]. DIAP2 is required to sustain AMP expression in Drosophila S2 cells. However, the role of DIAP2 is limited to the IMD signaling, as DIAP2 null flies showed no defects in immune responses triggered via the Toll pathway, such as response against fungal infections [15][16][17][18]. Recently, it was reported that Gram-negative bacterial infections induce binding of DIAP2 to the caspase8 homolog DREDD, targeting it for polyubiquitination in a RING finger-dependent manner for Relish processing and subsequent AMP expression [19,20]. The functions of IAPs in defense against microbial infection and induction of NF-κB activity in mammals are evolutionarily conserved [7,8,[21][22][23][24]. For example, mammalian cIAP-1, cIAP-2, and XIAP expressions are induced by NF-κB and contribute to NF-κB-mediated protection of some cells against TNFα-induced apoptosis [7,22,24]. However, the function of IAP2 in NF-κB activation is still unclear in other invertebrates, except Drosophila.

2.1: Shrimp culture
Healthy Pacific white shrimp (L. vannamei), approximately 4-5 g in body weight, were obtained for gene cloning and tissue distribution analysis, and those approximately 1-2 g in body weight were used for dsRNA-mediated gene silencing. All shrimp were purchased from a local shrimp farm in Zhuhai, Guangdong Province, China. The shrimp were cultured in a recirculating water tank system containing air-pumped seawater (2.5% salinity) at 24-26 °C and fed commercial feed at 5% of body weight twice a day, as previously described [43]. The shrimp were cultured for at least seven days to facilitate acclimation before the experiments were conducted.

2.2: RNA extraction and cDNA synthesis
Total RNA was extracted from the gill of L. vannamei using an RNeasy Mini Kit (Qiagen, Germany). Residual genomic DNA was removed using RNase-free DNase I (Qiagen, Germany). The cDNA template for rapid amplification of cDNA ends (RACE) PCR was prepared using a SMARTer™ RACE cDNA Amplification Kit (Clontech, USA). For gene cloning, firststrand cDNA was prepared using a PrimeScript™ 1st strand cDNA Synthesis Kit (Takara Bio, China). For the real-time quantitative PCR (qPCR) analysis, first-strand cDNA was prepared using a PrimeScript™ RT Reagent Kit (Takara Bio, China). cDNA of LvIAP1-3 were obtained using 5′-and 3'-RACE approach, as described in our previous studies [44][45][46].

Primer
Primer sequence (5'-3') cDNA cloning .1LvIAP3-F GCTCTAGACTTTGGAATATTACCAACTGGTTTTC * T7 RNA polymerase binding site is underlined; ** primers used in the cellular localization and luciferase reporter assays were the same.

2.8: Cell culture
Because no immortalized shrimp cell line is currently available, Drosophila Schneider 2 (S2) cells (Invitrogen), derived from a macrophage-like lineage, were used to analyze the cellular localization and function of LvIAP1-3. Drosophila S2 cells were maintained at 28 °C in Schneider's Drosophila medium (SDM) (Invitrogen) without CO 2 and supplemented with 10% fetal bovine serum (FBS). When the culture density reached 6-20 × 10 6 viable cells ml −1 , the Drosophila S2 cells were passaged onto a new plate at a density of 5 × 10 5 viable cells ml −1 .

2.9: Cellular localization analysis
Drosophila S2 cells were seeded onto poly-l-lysine-treated coverslips in 24-well plates at 24 hours before transfection. pAc5.1-LvIAP1-3-GFP were transfected into Drosophila S2 cells using Effectene Transfection Reagent (Qiagen, Germany) according to the manufacturer's protocol. Thirty-six hours after transfection, the cells on the coverslips were washed twice with PBS, fixed in Immunol Staining Fix Solution (Beyotime, China) and stained with Hoechst 33258 (Beyotime, China). The coverslips were subsequently examined for protein cellular localization using a Leica laser scanning confocal microscope as previously described [45][46][47].

2.10: Dual luciferase reporter assays
Drosophila S2 cells were seeded onto a 96-well culture plates in 100 µl medium at 2 × 10 5 cells ml −1 for 24 hours prior to transfection. To examine whether LvIAP2 affects the promoter activities of NF-κB-controlled AMPs, the expression vector pAC5.1-LvIAP2 (0.05 µg per well) was cotransfected with the luciferase reporter gene pGL3-Basic, pGL3-PEN453, pGL3-PEN309, pGL3-PEN4, pGL3-Drs or pGL3-AttA (0.05 µg per well) as described in our previous studies [44,47]. The pRL-TK Renilla luciferase vector was used as an internal control. The cells were harvested and lysed at 36 hours after transfection to examine luciferase activities using the Dual-Luciferase Reporter Assay System (Promega, USA).

2.11: Preparation of dsRNA and gene silencing through dsRNA injection in vivo
The double-stranded RNAs (dsRNAs) of LvIAP1-3 and GFP (were prepared using T7 RiboMAX Express Kit (Promega, USA) as previous described [43]. Briefly, DNA templates for the production of dsLvIAP1-3 and dsGFP were PCR amplified using gene-specific primers with the T7 RNA polymerase binding site at the 5' terminus to produce sense and anti-sense RNA strands separately. The single-stranded RNA was annealed to generate dsRNA. After purification, the dsRNA was quantified and stored at -80° C. For the dsRNA-mediated gene silencing experiments, the experimental group (1-2 g per shrimp) was treated with dsLvIAP1, dsLvIAP2 or dsLvIAP3 (1 µg/g shrimp) through intramuscular injection, while the control groups were injected with dsGFP and PBS, respectively. To determine the silencing effects, the gill samples from at least three shrimp from each treatment were collected at 0, 24, 72, 120, and 144 hours post-dsRNA injection (hpi), and the total RNA was extracted. The total RNA from the gills of dsRNAinjected L. vannamei was reverse-transcribed into the firststrand cDNA to assess the gene silence efficiency. For LvIAP2, the hemocytes were collected to assess the gene silencing efficiency because we did not observe an obvious reduction in gene expression in the gill of dsLvIAP2-injected shrimps.

2.13: The WSSV infection experiments in dsRNAinjected L. vannamei
The efficiency of gene silencing in dsLvIAP1-and dsLvIAP3injected L. vannamei was significant compared with that of the control groups (> 80%) at all examined time points selected for qPCR analysis. In the WSSV infection experiments, L. vannamei were intramuscularly infected with a WSSV inoculum (approximately 10 7 copies/shrimp) at 48 hours after dsRNA injection and the gills were collected at 0, 3, 6, 12, 24, 36, and 48 hpi to assess WSSV VP 28 expression.

2.14: Statistical analyses
The data are presented as the means ± standard error of the mean (SEM). Student's t-test was used to compare the means of two samples using Microsoft Excel. The chi-square statistical analysis was performed to assess differences in the mortality rates through a comparison of the mortality of the dsLvIAP2 injection group with that of the PBS or dsGFP-injected group. In all cases, the differences were considered statistically significant at p < 0.05 and highly significant at p < 0.01.

3.1: Cloning and sequence analysis of LvIAP1-3, Lvlysozyme, Lvcrustin1-3, LvALF1-3, and LvVICP1-2
Based on the EST sequences of L. vannamei in the NCBI database, the full-length cDNAs of three novel L. vannamei IAPs (LvIAP1-3) were cloned. LvIAP1 cDNA was 879 bp with an ORF of 420 bp, encoding a putative protein of 139 amino acids, a 5' untranslated region of 79 bp, and a 3' untranslated region of 380 bp ( Figure 1A). LvIAP2 cDNA was 3, 166 bp with an ORF of 2,100 bp, encoding a putative protein of 699 amino acids, a 5' untranslated region of 593 bp, and a 3' untranslated region of 473 bp ( Figure 1B). LvIAP3 cDNA was 2, 219 bp with an ORF of 1,176 bp, encoding a putative protein of 496 amino acids, a 5' untranslated region of 59 bp, and a 3' untranslated region of 399 bp ( Figure 1C).
LvIAP1 contains one BIR domain and shares 38% and 29% identities to human survivin and Drosophila Deterin, respectively ( Figure 1D). LvIAP2 contains three BIR domains and a C-terminal RING domain, and is 27% and 30% identical to Drosophila IAP1 and IAP2, respectively ( Figure 1D). LvIAP3 is a completely novel member of the IAP family proteins, possessing two BIR domains, and it is not similar to any known IAPs ( Figure 1D).
To investigate the regulation of shrimp AMPs through LvIAP2 in vivo, one novel Lvlysozyme, three novel Lvcrustins, three novel LvALFs, and two novel LvVICPs were cloned. LvVICPs (Vibrio penaeicidae-induced cysteine and proline-rich peptides) are homologs of Stylicins in Pacific blue shrimp Litopenaeus stylirostris, which are new members of the recently identified shrimp AMPs with strong antifungal activity against Fusarium oxysporum, a pathogenic fungus of shrimp. The sequences of Lvlysozyme, Lvcrustin1-3, LvALF1-3, and LvVICP1-2 are provided in Figure S2.

3.2: Phylogenetic tree construction
Using MEGA 4.0 software, we constructed NJ phylogenetic trees for IAPs from typical species. The NJ phylogenetic tree revealed two groups of shrimp IAPs: LvIAP1 and LvIAP3 were clustered with Dmdeterin and Hssurvivin in one group, and LvIAP2 clustered with DmIAP2 in another group (Figure 2).

3.4: Expression profiles of LvIAP1-3 after microbial challenge
After WSSV infection, LvIAP1 was upregulated in the gill, hemocytes, and intestine compared with the PBS-injected group ( Figure 4A-D); LvIAP2 was also upregulated in the gill, hemocytes, and hepatopancreas ( Figure 4F-H); but LvIAP3 was only slightly upregulated in the gill and intestine ( Figure 4I-

3.5: Cellular localization of LvIAP1-3 in Drosophila S2 cells
To examine the cellular localization of LvIAP1-3, LvIAP1, LvIAP2, and LvIAP3 were fused to GFP using a pAc5.1-N-GPF vector and expression of fusion proteins were observed using confocal microscopy. Both LvIAP1 and LvIAP3 fusion proteins were widely distributed in the cytoplasm and nucleus of Drosophila S2 cells, whereas LvIAP2 was distributed in the cytoplasm but appeared as speck-like aggregates in the nucleus ( Figure 6).

3.6: The reduced expression of LvIAP1-3 in vivo by dsRNA-mediated gene silencing
To investigate the function of LvIAP1-3 in shrimp defense against WSSV infection, dsRNA-mediated gene silencing experiments were performed. dsLvIAP1-3 (1 µg/g shrimp) were intramuscularly injected into shrimp separately, in the experimental groups, while injection of dsGFP or PBS was used in the control groups. In the gill, the expression of LvIAP1 and LvIAP3 was significantly suppressed at 24, 72, 120 and 144 hpi (Figure 7), while the expression of LvIAP2 was silenced in hemocytes, but not in the gill ( Figure 8A). Intriguingly, the LvIAP2-silenced shrimp died within 48 hours after dsLvIAP2 injection ( Figure 8B).

Figure 8. Silencing of LvIAP1 and LvIAP3 facilitates the reproduction of WSSV.
At 48 hours after dsLvIAP1, dsLvIAP3, dsGFP or PBS injection, the shrimp were infected intramuscularly with a WSSV inoculum (107 copies/shrimp). At the indicated time points after WSSV infection, the gills of these shrimp were collected for qPCR analysis. The mRNA expression level of WSSV VP28 in the gills of shrimp injected with PBS, dsGFP (control), dsLvIAP1, or dsLvIAP3 after WSSV infection were determined using qPCR. The mRNA expression level of WSSV VP28 was normalized to that of LvEF-1α using the relative standard curve method for calculation of changes in gene expression as described in previous studies [43]..  The cumulative mortality rate of shrimp injected with dsGFP (control) or dsLvIAP2. The chi-square statistic was calculated to assess the differences in mortality rates by comparing the mortality of dsLvIAP2-injection group with that of the dsGFP-injection group (***p < 0.001). doi: 10.1371/journal.pone.0072592.g009

3.7: WSSV VP28 expression in dsRNA-injected L. vannamei
To further evaluate the role of LvIAP1 and LvIAP3 in shrimp defense against WSSV infection, we performed WSSV infection experiments in dsRNA-injected L. vannamei. At 48 hours after dsRNA injection, L. vannamei were infected with WSSV. We observed that at 24, 36 and 48 hpi, the expression of WSSV VP28 in the gill of the dsLvIAP1-and dsLvIAP3injected groups was dramatically higher than that in the dsGFP-or PBS-injected group (Figure 9). At 24 hpi, the expression of VP28 was low in the PBS and dsGFP-injected groups, but in the dsLvIAP1-and dsLvIAP3-injected groups, the expression of VP28 was high, suggesting that the silencing of LvIAP1 and LvIAP3 accelerates WSSV infection (Figure 9). We also observed that at 24 and 36 hpi, the expression of WSSV VP28 was higher in LvIAP1-silenced shrimp that in LvIAP3 silenced shrimp (Figure 9). In LvIAP1-silenced shrimp, WSSV VP28 was gradually increased, but in LvIAP3-silenced shrimp, the expression of WSSV VP28 diminished (Figure 9). These results suggest that LvIAP1 and LvIAP3 are involved in the host defense against WSSV infection differently.

3.8: The activation of the promoters of NF-κB pathwaycontrolled AMPs by LvIAP2 in Drosophila S2 cells
A comparison with four Drosophila IAPs (DIAPs) revealed that LvIAP2 is similar to DIAP1 and DIAP2 in domain structure and protein sequence ( Figure 1D). DIAP1 plays an essential role in regulation of apoptosis, and DIAP2 is required for the IMD pathway in AMP regulation but is dispensable for Drosophila survival [16,53]. A previous study indicated that a shrimp IAP homolog of LvIAP2 evaluated in this study is essential for shrimp survival [42]. In this study, we investigated whether LvIAP2 functions in AMP regulation through the IMDmediated NF-κB pathway in Drosophila S2 cells. The results of the dual luciferase reporter assays indicated that overexpression of LvIAP2 significantly induced the promoter activities of Drosophila AMPs, including Drosomycin (Drs) (5.57-fold) and Attacin A (AttA) (2.06-fold), P. monodon AMP Penaeidin (PEN309 and PEN453 at 3.76 and 4.47-fold, respectively), and L. vannamei AMP Penaeidin4 (PEN4) (4.22fold) ( Figure 10). However, overexpression of neither LvIAP1 nor LvIAP3 affected the activities of these AMP promoters (result not shown).

3.9: The activation of the promoters of WSSV069, WSSV303, and WSSV371 by LvIAP2 in Drosophila S2 cells
In a previous study, we showed that several viral genes, including WSSV069, WSSV303, and WSSV371 that possess NF-κB binding sites in the promoter regions, were regulated through the NF-κB signaling pathway [48]. Here, we also showed that overexpression of LvIAP2 in Drosophila S2 cells activatedthe promoters of WSSV069 (ie1), WSSV303, and WSSV371 by 2.27-, 1.79-, and 3.30-fold, respectively ( Figure  11).

Discussion
Apoptosis is a tightly regulated process in which excess or damaged cells are eliminated to maintain tissue homeostasis [1,3,6,21]. Apoptosis is also a major defense mechanism to remove unwanted and potentially dangerous cells, such as virus-infected cells [3,5,54,55]. Shrimps use apoptosis in defense against WSSV infection, and WSSV encodes two antiapoptosis proteins, AAP-1 (ORF390 or WSSV449) and WSSV222, to subvert host apoptosis responses to facilitate viral replication [26,27,29,39]. Inhibitors of apoptosis proteins (IAPs) inhibit the activity of caspases, the primary executor of the apoptosis program, and play important roles in regulating the progression of apoptosis from insects to humans [1,6,56]. In addition to apoptosis regulation, IAPs also participate in diverse cellular activities, such as signal transduction, innate immunity, and mitosis [21,57,58]. In this study, three IAPs from L. vannamei (LvIAP1-3) were cloned and characterized. Using dsRNA-mediated gene silencing, we investigated the functions of IAPs in WSSV infection and shrimp AMP regulation. LvIAP1-3 mRNAs were primarily expressed in the muscle and upregulated after WSSV infection (Figures 3-5). After WSSV infection, LvIAP1 was upregulated in the gill, hepatopancreas, hemocytes, and intestine ( Figure 4); LvIAP2 was upregulated in the gill, hepatopancreas, hemocytes, but not in the intestine ( Figure 4); LvIAP3 did not show significant changes (Figure 4). In LvIAP1-or LvIAP3-silenced shrimp, the expression of WSSV VP28 increased dramatically compared with that in the dsGFP control group (Figure 9), suggesting protective roles of LvIAP1 and LvIAP3 in shrimp defense against WSSV infection. In the present study, dsLvIAP1 and dsLvIAP3 were injected followed by WSSV infection. The silencing of LvIAP1 and LvIAP3 in the early stages during WSSV infection might promote apoptosis to facilitate the spread of virus progeny to neighboring cells. However, the detailed mechanism underlying this process needs further investigation (e.g., silencing LvIAP1 and LvIAP3 at different stages during WSSV infection and observing the replication of WSSV). Interestingly, LvIAP2 was only effectively silenced in the hemocytes, but not in the gill, and the LvIAP2-silenced shrimp died within 48 hours after dsLvIAP2 injection ( Figure 8). This phenomenon was also observed in a recently published paper, in which the authors concluded that reduction in the number of hemocytes in IAP2-silenced shrimp reflects extensive apoptosis [42]. We also observed that the circulating hemocytes were dramatically reduced in LvIAP2-silenced shrimp (results not shown). Thus, hemocytes play a pivotal role in shrimp survival, and LvIAP2 plays a central role in regulation of shrimp hemocyte apoptosis. LvIAPs were also cloned in a recent report [42] and the function of LvIAP2 in shrimp haemocyte apoptosis is well studied. In this study, we investigated induced expression of LvIAP1-3 by WSSV infection and their potential involvements in host defense against viral infection. Particularly, we further studied the function of LvIAP2 in regulation of shrimp AMPs.
A comparison with four Drosophila IAPs (DIAPs) revealed that LvIAP2 is structurally related to DIAP1 and DIAP2 and is most similar to DIAP2 (Figure 1). DIAP1 is essential for Drosophila cell survival in vivo and in vitro, whereas DIAP2 is required for the IMD pathway in AMP regulation, but is dispensable for Drosophila survival [16,53]. In the present study, we observed that, similar to DIAP2, LvIAP2 activated the IMD pathway through the induction of the promoter activities of Drosophila and shrimp AMPs in Drosophila S2 cells ( Figure  10). In addition, shrimp AMPs, such as PENs, lysozyme, crustins, VICPs, and ALFs, were significantly downregulated in the hemocytes of LvIAP2-silenced shrimp ( Figure 12). The increase expression of ALFs might reflect different regulation mechanisms of various AMPs, which has also been recently observed in other studies [59]. The silencing of Cactus (a shrimp IκB homolog and potential negative regulator of the shrimp Toll pathway) in Chinese shrimp Fenneropenaeus chinensis downregulated ALF expression, consistent with the upregulation of ALF expression in the hemocytes of LvIAP2silenced L. vannamei [59]. The silencing of LvTollip, a potential negative regulator of the shrimp Toll pathway, also downregulates the expression of another shrimp AMP, PEN2 [60]. These results suggest that shrimp AMPs are regulated through the Toll/IMD-NF-κB signaling pathway, but with different mechanisms. We propose that ALFs might have different regulation mechanisms from those of PENs, lysozyme, crustins, and VICPs.
In the present study, we cloned two new members of the recently identified shrimp AMP VICPs (Vibrio penaeicidaeinduced cysteine and proline-rich peptide, called Stylicins in Pacific blue shrimp Litopenaeus stylirostris) [61]. Litopenaeus stylirostris Stylicin displays strong antifungal activity against Fusarium oxysporum, a pathogenic fungus of shrimp. The regulation of LvVICPs through LvIAP2 might suggest that the shrimp IMD pathway is involved in antifungal responses. In Drosophila, the Toll pathway, but not the IMD pathway, primarily regulates antifungal and anti-Gram-positive bacterial responses [10,11]. Thus, the antibacterial and antifungal mechanisms might be different in the Toll and IMD pathways in Drosophila and shrimps. Notably, the expression of all the ALFs, including LvALF1, LvALF2, and LvALF3, was upregulated in the hemocytes of LvIAP2-silenced shrimp. Thus, LvIAP2 might negatively regulate the expression of ALFs.
Although LvIAP1-3 possess the characteristic baculoviral IAP repeat (BIR) domain, these proteins also differed in many aspects. LvIAP1 has one BIR domain, similar to mammalian survivin and Drosophila deterin, whereas LvIAP2 contains three BIR domains and a C-terminal RING domain. Therefore, LvIAP2 is structurally similar to mammalian XIAP, cIAP1, and cIAP2 and Drosophila IAP2 ( Figure 1D), which possess three BIR domains and a RING domain and are involved in NF-κB activation [7,8,[21][22][23][24]. LvIAP3 is a completely novel member of the IAP family proteins, with two BIR domains, which is not similar to any known mammalian or insect IAPs. Our results suggest that LvIAP2 possesses dual functions in both the DIAP1-mediated apoptosis and DIAP2-mediated NF-κB activation of the IMD pathway [41,42]. Considering the protein identity and domain structure of LvIAP2 and biological function in AMP regulation by LvIAP2, we propose that LvIAP2 is the homolog of DIAP2, but not DIAP1. Therefore, we refer to this molecule as LvIAP2 in the present study.
Apoptosis-related genes, such as Pmcaspase, have been targets of small molecule drugs to improve the apoptotic activity of shrimp hemocytes for the inhibition of WSSV infection [27,62]. Thus, in future studies, the detailed functions of shrimp IAPs in different stages during WSSV infection should be investigated to provide information for the development of drugs targeting shrimp IAPs to manipulate apoptosis as novel strategies for the prevention and control of WSSV infection. Figure S1. The promoter sequences (shaded regions) of Drosophila Attacin A (AttA), Drosomycin (Drs), Litopenaeus vannamei Penaeidin4, and Penaeus monodon penaeidin (two types, PmPEN309 and PmPEN453) were shown. The primers used in luciferase reporter construction were also provided. Protocols for dual luciferase reporter assays are as followings: 1) Drosophila S2 cells were maintained at 28°C in standard Drosophila medium (Serum-Free Medium; Invitrogen, USA), supplemented with 10% fetal bovine serum (FBS) and 1% Penicillin-Streptomycin solution.