TmSpz6 Is Essential for Regulating the Immune Response to Escherichia coli and Staphylococcus aureus Infection in Tenebrio molitor

Spätzle is an extracellular protein that activates the Toll receptor during embryogenesis and immune responses in Drosophila. However, the functions of the spätzle proteins in the innate immune response against bacteria or fungi in T. molitor are not well understood. Therefore, in this study, the open reading frame (ORF) of TmSpz6 was identified and its function in the response to bacterial and fungal infections in T. molitor was investigated using RNAi. The highest expression of TmSpz6 was in prepupae, and 3- and 6-day-old pupae, while remarkable expression was also observed in other stages. The tissue-specific expression analysis showed that TmSpz6 expression was highest in the hemocytes of larvae. TmSpz6 expression was highly induced when challenged with Escherichia coli, Staphylococcus aureus, or Candida albicans at 6 h post-injection; however, TmSpz6-silenced larvae were significantly more susceptible to only E. coli and S. aureus infection. The antimicrobial peptides (AMPs) gene expression analysis results show that TmSpz6 mainly positively regulated the expression of TmTencin-2 and -3 in response to E. coli and S. aureus infection. Collectively, these results suggest that TmSpz6 plays an important role in regulating AMP expression and increases the survival of T. molitor against E. coli and S. aureus.


Introduction
Insects have well-developed and complex innate immune systems that are divided into humoral and cellular components. The humoral immune system principally consists of antimicrobial peptides (AMPs), lectins, lysozyme, protease inhibitors, and other factors [1]. The recognition of invading pathogens leads to the activation of signal transduction pathways, such as Toll or immune deficiency (IMD), and ultimately induces the expression of antimicrobial peptides (AMPs) that attack the invading pathogens [2,3].
In Drosophila, AMP production is controlled by downstream signal transduction pathway that includes spätzle, Toll, tube, pelle, and cactus [4][5][6][7]. This pathway is activated when pattern-recognition receptors (PRRs) recognize the pathogen-associated molecular pattern [8] and convey the signal to a Insects 2020, 11, 105 2 of 15 proteolytic cascade that leads to the cleavage of the cytokine-like protein pro-spätzle; the resulting cleaved, mature spätzle activates the Toll receptor as a ligand [9,10].
Binding of spätzle to the Toll receptor activates a downstream signaling pathway containing several protein complexes, including adaptor proteins such as myeloid differentiation primary response 88 (MyD88), Tube, and the serine-threonine innate immunity kinase (Pelle) [11]. Signaling through the MyD88-Tube-Pelle complex leads to the phosphorylation and degradation of the IκB factor Cactus, which inhibits the nuclear localization and activity of NF-κB transcription factors. Once Cactus is degraded, both Dorsal and Dif translocate to the nucleus and bind to κB-related sequences in the AMP genes [12].
Initially, spätzle exists as an inactive extracellular pro-spätzle, which contains a signal peptide, an N-terminal regulatory cleavage site, and a signaling precursor consisting of a 106-amino acid C-terminal active fragment [13,14]. The active ligand spätzle is generated during development or immune response [14].
Spätzle proteins have been shown to be important in the innate immune response to microbial infection in various arthropods from insects to shrimp. However, apart from a biochemical characterization [9], the functions of the spätzle genes in the T. molitor immune system in response to microbial challenge have not been yet studied. Therefore, the current study focused on the identification and functional characterization of TmSpätzle 6 in innate immune response to various pathogens in T. molitor.

Insect Culture
T. molitor (mealworm) was maintained at 27 ± 1 • C and 60 ± 5% relative humidity in the dark on an artificial diet containing 170 g of whole-wheat flour, 20 g of fried bean powder, 10 g of soy protein, 100 g of wheat bran, 200 mL of sterile water, 0.5 g of chloramphenicol, 0.5 g of sorbic acid, and 0.5 mL of propionic acid. For the experiments, 10th-12th instar larvae were used. To ensure that uniformly sized larvae were used, the larvae were separated according to size using a set of laboratory test sieves (Pascall Eng. Co., Ltd., Crawley, Sussex, England).

Preparation of Microorganisms
The gram-negative bacterium Escherichia coli K12, the gram-positive bacterium Staphylococcus aureus RN4220, and the fungus Candida albicans were used to study the function of TmSpz6 in the innate immune response of mealworms against microbial infection. These microorganisms have been repeatedly used by various researchers to study the immune related gene expression [24][25][26]. The microorganisms were cultured in Luria-Bertani (LB; E. coli and S. aureus) and Sabouraud dextrose (C. albicans) broths at 37 • C overnight and were subsequently subcultured at 37 • C for 3 h. Then, the microorganisms were harvested and washed two times by centrifugation at 3500 rpm for 10 min in phosphate-buffered saline (PBS; pH 7.0). The washed microorganisms were suspended in PBS and their optical densities were measured at 600 nm (OD 600 ) to determine the concentration. Finally, 10 6 cells/µL of E. coli or S. aureus and 5 × 10 4 cells/µL of C. albicans were separately injected into the larvae.

Identification and Cloning of the Full-length TmSpz6 cDNA
The T. molitor TmSpz6 gene was identified by a local-tBLASTn analysis using the amino acid sequence of the T. castaneum spz6 gene (NP_001164082.1) as the query. The partial cDNA sequence of Tmspz6 was obtained from the T. molitor RNAseq database, and the full-length cDNA sequence of TmSpz6 was identified by the 5 -and 3 -rapid amplification of cDNA end (RACE) polymerase chain reaction (PCR) using a SMARTer RACE cDNA amplification kit (Clontech, Mountain View, CA, USA) according to the manufacturer's instructions. The PCR was performed with AccuPower ® PyroHotStart Taq PCR PreMix (Bioneer, Korea) and TmSpz6-specific primers (TmSpz6-cloning_Fw and TmSpz6-cloning_Rv; Table 1) under the following cycling conditions: a pre-denaturation step at 95 • C for 5 min, followed by 35 cycles of denaturation at 95 • C for 30 s, annealing at 53 • C for 30 s, and extension at 72 • C for 2 min, with a final extension step at 72 • C for 5 min on a MyGenie96 Thermal Block (Bioneer, Korea). The PCR products were purified using the AccuPrep ® PCR Purification Kit (Bioneer, Korea), immediately ligated into T-Blunt vectors (Solgent, Korea), and transformed into E. coli DH5α competent cells according to the manufacturer's instructions. Plasmid DNA was extracted from the transformed cells using the AccuPrep ® Nano-Plus Plasmid Extraction Kit (Bioneer, Korea), sequenced, and analyzed. Finally, the full-length cDNA sequence of TmSpz6 was obtained.

Domain and Phylogenetic Analyses
Specific domains were analyzed using the InterProScan 5 and BLASTp programs. A multiple sequence alignment was performed with representative Spz6 protein sequences from other insects obtained from GenBank using ClustalX2 software. Phylogenetic and percentage identity analyses were conducted using ClustalX2 and MEGA 7 programs.
The samples were collected into 500 µL of guanidine thiocyanate RNA lysis buffer (2 mL of 0.5 M EDTA, 1 mL of 1 M MES Buffer, 17.72 g of guanidine thiocyanate, 0.58 g of sodium chloride, 0.7 mg of phenol red, 25 µL of Tween-80, 250 µL of glacial acetic acid, and 500 µL of isoamyl alcohol) and were homogenized with a homogenizer (Bertin Technologies, France) at 7500 rpm for 20 s. The total RNA was extracted using the modified LogSpin RNA isolation method [27], and 2 µg of the extracted total RNA was used to immediately synthesize cDNA with AccuPower ® RT PreMix (Bioneer, Korea) and Oligo (dT) 12-18 primers on a MyGenie96 Thermal Block (Bioneer, Korea) according to the manufacturer's instructions.
Real-Time Quantitative PCR (RT-qPCR) was performed on an Exicycler TM 96 Real-Time Quantitative Thermal Block (Bioneer, Daejeon, Korea) with gene-specific primers under the following cycling conditions: an initial denaturation step at 94 • C for 5 min, followed by 45 cycles of denaturation at 95 • C for 15 s and annealing at 60 • C for 30 s. The 2 −∆∆Ct method [28] was used to analyze TmSpz6 expression levels. T. molitor ribosomal protein L27a (TmL27a) was used as an internal control to normalize differences in template concentration between samples.

RNA Interference Analysis
To synthesize the double-stranded (ds) RNA of the TmSpz6 gene, primers containing the T7 promoter sequence at their 5 ends were designed using SnapDragon-Long dsRNA design software ( Table 1). The PCR was conducted using AccuPower ® Pfu PCR PreMix with the TmSpz6_Fw and TmSpz6_Rv primers (Table 1) under the following cycling conditions: an initial denaturation step at 94 • C for 2 min followed by 35 cycles of denaturation at 94 • C for 30 s, annealing at 53 • C for 30 s, and extension at 72 • C for 30 s, with a final extension step at 72 • C for 5 min. PCR products were purified using the AccuPrep PCR Purification Kit (Bioneer, Daejeon, Korea), and dsRNA was synthesized using the Ampliscribe TM T7-Flash TM Transcription Kit (Epicentre Biotechnologies, Madison, WI, USA) according to the manufacturer's instructions. After synthesis, the dsRNA was purified by precipitation with 5 M ammonium acetate and 80% ethanol, and then it was quantified with an Epoch spectrophotometer (BioTek Instruments, Inc., Winooski, VT, USA). The dsRNA for enhanced green fluorescent protein (dsEGFP) was synthesized for use as a control and was stored at −20 • C until use.

Effect of TmSpz6 Gene Silencing on the Response to Microorganism Challenge
To study the importance of TmSpz6 in the T. molitor immune response, dsTmSpz6 (1 µg/µL) was first injected into young-instar larvae (10th-12th instars; n = 30) using disposable needles mounted onto a micro-applicator (Picospiritzer III Micro Dispense System; Parker Hannifin, Hollis, NH, USA). An equal amount of dsEGFP was injected in similar larvae as a negative control. TmSpz6 knockdown was evaluated, and over 90% knockdown was achieved at 2 days post-injection. Second, the TmSpz6-silenced and dsEGFP-injected larval groups were challenged with E. coli (10 6 cells/µL), S. aureus (10 6 cells/µL), or C. albicans (5 × 10 4 cells/µL) in triplicate experiments. The challenged larvae were maintained for 10 days, during which the number of surviving larvae were recorded. The survival rates of the TmSpz6-silenced larvae were compared to survival of control larvae.

Effect of dsTmSpz6 on AMP Expression in Response to Microbial Challenge
To characterize the function of TmSpz6 in regulating AMP gene expression in response to microbial infection, TmSpz6 gene expression in larvae was silenced with RNAi and then these larvae were injected with microorganisms (E. coli, S. aureus, or C. albicans). dsEGFP and PBS were used as the negative and injection controls, respectively. At 24 h post-injection, the hemocytes, fat body, and gut were dissected, and then total RNA was extracted from these tissues and cDNA was synthesized as described above. Next, qRT-PCR was conducted using specific primers (Table 1) to analyze the temporal expression patterns of 14 AMP genes: TmTencin-1 (TmTen-1), TmTencin-2 (TmTen2), TmColeoptericin-2 (TmCol-2), TmCecropin-2 (TmCec-2), TmThaumatin like protein-1 (TmTLP-1), and TmThaumatin like protein-2 (TmTLP-2).

Data Analysis
Statistical analyses were conducted using SAS 9.4 software (SAS Institute, Inc., Cary, NC, USA), and cumulative survival was analyzed by Tukey's multiple test, at a significance level of p < 0.05. AMP gene expression was calculated using the delta Ct (∆∆Ct) method, and the fold change compared to the internal control (TmL27a) and external control (PBS) was calculated by the 2 (∆∆Ct) method.

Sequence Identification and Phylogenetic Analysis of TmSpz6
The full-length open reading frame (ORF) sequence of TmSpz6 was obtained from the T. molitor RNAseq database and by 5 -and 3 -RACE PCR. The TmSp6 ORF is 1227 bp and encodes 408 amino acid residues (Figure 1). Domain analysis indicated that TmSpz6 contains one cystine-knot domain at the C-terminus, one cleavage site, and one signal peptide region. Phylogenetic analysis revealed that TmSpz6 grouped together with another spätzle 6 from a Coleopteran insect (Tribolium castaneum spätzle 6) ( Figure 2).

Developmental and Tissue-Specific Expression Patterns of TmSpz6
The developmental and tissue-specific expression patterns of TmSpz6 mRNA were examined by RT-qPCR. TmSpz6 transcripts were observed in all tested developmental stages and tissues ( Figure 3). TmSpz6 was expressed at similar levels in young and late larvae, but was highly expressed in pre-pupae. Expression was decreased in 1-and 2-day-old pupae but was then highly upregulated and peaked in 3-day-old pupae. This was followed by a gradual decrease in expression in 4-and 5-day-old pupae and an increase in 6-day-old pupae. During the adult stage, TmSpz6 was expressed at similar levels at all examined ages, except it was slightly lower in 5-day-old adults ( Figure 3A). Insects 2020, 11, x FOR PEER REVIEW 6 of 15

Developmental and Tissue-Specific Expression Patterns of TmSpz6
The developmental and tissue-specific expression patterns of TmSpz6 mRNA were examined by RT-qPCR. TmSpz6 transcripts were observed in all tested developmental stages and tissues ( Figure  3). TmSpz6 was expressed at similar levels in young and late larvae, but was highly expressed in prepupae. Expression was decreased in 1-and 2-day-old pupae but was then highly upregulated and similar levels at all examined ages, except it was slightly lower in 5-day-old adults ( Figure 3A). The examination of different tissues revealed that TmSpz6 was highly expressed in hemocytes, but was expressed at lower levels in the integument, fat body, and Malpighian tubules of late instar larvae ( Figure 3B). In adults, expression was high in the integument and fat body followed by the testis and hemocytes ( Figure 3C). Comparatively low TmSpz6 expression levels were detected in the gut, Malpighian tubules, and ovaries of 5-day-old adults. The results indicate that TmSpz6 expression gradually increased from the young larval to prepupal stage. In the pupal stage, the highest expression was observed in 4-day-old pupae. In adults, there was no considerable difference in expression in 2-5-day-old adults. The tissue-specific expression patterns of TmSpz6 were also assessed in late larvae (B) and 5-day-old adults (C). The hemocytes (HC), gut, fat body (FB), Malpighian tubules (MT), and integument (INT) (for late instar larvae and adults), as well as the testes (TE) and ovaries (OV) (for adults), were dissected and collected from 20 late larvae and 5-day-old adults. T. molitor 60S ribosomal protein L27a (TmL27a) served as an endogenous control to normalize RNA levels between samples. The data are the means of three biological replicates. The asterisks indicate significant differences (p ≤ 0.05).

Temporal Induction of TmSpz6 after Microbial Challenge
To determine the inducibility of TmSpz6 during microbial infection, the temporal expression of TmSpz6 in T. molitor larvae was examined after injecting E. coli, S. aureus, or C. albicans. The temporal expression patterns in three immune-related tissues, hemocytes, fat body, and gut, were analyzed at 3, 6, 9, 12, and 24 h post-injection by RT-qPCR. The microbial challenge time-dependently induced transcription of TmSpz6 in all tested tissues. All injected microorganisms induced the highest TmSpz6 expression in hemocytes at 6-h post injection ( Figure 4A). In E. coli-and S. aureus-injected larvae, the highest TmSpz6 expression in the gut was observed at 9 h post injection ( Figure 4B), whereas in E. TmSpz6 expression patterns across the developmental stages of T. molitor, including, young larvae (YL), late larvae (LL), pre-pupa (PP), 1-7-day-old pupae (P1-7), and 1-5-day-old adults (A1-5) were examined (A). For each sample, RNA extracted from 20 individuals was used to synthesis cDNA. The results indicate that TmSpz6 expression gradually increased from the young larval to pre-pupal stage. In the pupal stage, the highest expression was observed in 4-day-old pupae. In adults, there was no considerable difference in expression in 2-5-day-old adults. The tissue-specific expression patterns of TmSpz6 were also assessed in late larvae (B) and 5-day-old adults (C). The hemocytes (HC), gut, fat body (FB), Malpighian tubules (MT), and integument (INT) (for late instar larvae and adults), as well as the testes (TE) and ovaries (OV) (for adults), were dissected and collected from 20 late larvae and 5-day-old adults. T. molitor 60S ribosomal protein L27a (TmL27a) served as an endogenous control to normalize RNA levels between samples. The data are the means of three biological replicates. The asterisks indicate significant differences (p ≤ 0.05).
The examination of different tissues revealed that TmSpz6 was highly expressed in hemocytes, but was expressed at lower levels in the integument, fat body, and Malpighian tubules of late instar larvae ( Figure 3B). In adults, expression was high in the integument and fat body followed by the testis and hemocytes ( Figure 3C). Comparatively low TmSpz6 expression levels were detected in the gut, Malpighian tubules, and ovaries of 5-day-old adults.

Temporal Induction of TmSpz6 after Microbial Challenge
To determine the inducibility of TmSpz6 during microbial infection, the temporal expression of TmSpz6 in T. molitor larvae was examined after injecting E. coli, S. aureus, or C. albicans. The temporal expression patterns in three immune-related tissues, hemocytes, fat body, and gut, were analyzed at 3, 6, 9, 12, and 24 h post-injection by RT-qPCR. The microbial challenge time-dependently induced transcription of TmSpz6 in all tested tissues. All injected microorganisms induced the highest TmSpz6 expression in hemocytes at 6-h post injection ( Figure 4A). In E. coliand S. aureus-injected larvae, the highest TmSpz6 expression in the gut was observed at 9 h post injection ( Figure 4B), whereas in E. coliand C. albicans-injected larvae, the highest expression in the fat body was detected at 24 h post-injection ( Figure 4C).

Effect of TmSpz6 Silencing on T. molitor Survival
Since the temporal induction of TmSpz6 was observed following microorganism injection, the survival of TmSpz6-silenced T. molitor larvae in response to infection was assessed. The survival of TmSpz6-silenced or dsEGFP-injected T. molitor larvae after microbial injection was monitored for 10 days. The results show that the injection of dsTmSpz6 or dEGFP did not affect the survival of T. molitor larvae after injection with PBS. However, dsTmSpz6-injected larvae were highly susceptible to E. coli (68.5%) and S. aureus (57.5%) ( Figure 5B,C), whereas their survival rate after infection with C. albicans was not significantly different from that of the controls ( Figure 5D).

Effect of TmSpz6 Silencing on T. molitor Survival
Since the temporal induction of TmSpz6 was observed following microorganism injection, the survival of TmSpz6-silenced T. molitor larvae in response to infection was assessed. The survival of TmSpz6-silenced or dsEGFP-injected T. molitor larvae after microbial injection was monitored for 10 days. The results show that the injection of dsTmSpz6 or dEGFP did not affect the survival of T. molitor larvae after injection with PBS. However, dsTmSpz6-injected larvae were highly susceptible to E. coli (68.5%) and S. aureus (57.5%) ( Figure 5B,C), whereas their survival rate after infection with C. albicans was not significantly different from that of the controls ( Figure 5D).

Effects of TmSpz6 Gene Silencing on the Expression of AMP Genes
Based on the results of the survival study, the importance of TmSpz6 in the immune defense against gram-negative and gram-positive bacteria was postulated. Thus, the function of TmSpz6 in the production of AMPs in response to microbial infection was investigated by silencing the expression of TmSpz6 in T. molitor larvae, challenging them with E. coli, S. aureus, or C. albicans, and assessing the expression levels of 14 different AMP genes at 24 h post-infection.

Effects of TmSpz6 Gene Silencing on the Expression of AMP Genes
Based on the results of the survival study, the importance of TmSpz6 in the immune defense against gram-negative and gram-positive bacteria was postulated. Thus, the function of TmSpz6 in the production of AMPs in response to microbial infection was investigated by silencing the expression of TmSpz6 in T. molitor larvae, challenging them with E. coli, S. aureus, or C. albicans, and assessing the expression levels of 14 different AMP genes at 24 h post-infection.

Discussion
AMPs are essential effectors of the innate immune defense system against numerous pathogens [29,30]. In insects, the expression of AMPs is mainly regulated by the evolutionarily conserved Toll and IMD pathways [12]. Specifically, the Toll pathway, a well-known activator of AMP production in insects, is activated by the extracellular ligand spätzle [9]. The functions of the spätzle proteins in the innate immunity of various insect species have been repeatedly reported. In Drosophila, the most widely studied insect species, the functions of spätzle proteins in the defense response against microbial infections have been well studied [5,17,31]. The importance of spätzle in the activation of the Toll receptor and the subsequent activation of AMP production has also been studied in the lepidopteran insects, B. mori [32], and M. sexta [33].
In this study, TmSpz6 was identified in T. molitor and functionally characterized. TmSpz6 mRNA was highly expressed in the prepupal and pupal stages, whereas comparatively lower expression levels were observed in the larval and adult stages. Tissue-specific expression studies showed that TmSpz6 was expressed at various levels in all examined tissues in the larval and adult stages. The observed variations in TmSpz6 expression in different tissues and developmental stages is assumed to be controlled by developmental hormones. This assumption is based on previous studies demonstrating the importance of juvenile hormone (JH) and ecdysone in the insect innate immune response. For example, ecdysone was shown to activate PGRP-LC expression and induce AMP expression in Drosophila [34], JH was shown to act as an AMP-activator in B. mori [35], and ecdysone enhanced the B. mori immune system [36]. Therefore, it is possible that there are similar hormonal effects on TmSpz6 expression in T. molitor, caused by either ecdysone or other developmental hormones. Thus, the fluctuations in the expression of TmSpz6 at the same developmental stage or different stage are assumed to be due to hormonal changes. Briefly, the expression of TmSpz6 was highest at the perpupal stage and in 3-and 6-day-old pupae. These are transitional stages that the ecdysone commonly controls. The investigation of the expression of ecdysone during the development of Drosophila by radioimmune assay showed that ecdysone activity was highest during the pupal, prepupal, and late larval stages (in descending order) [37] In addition, TmSpz6 expression was highest in the hemocytes of larvae and adults. Previously, it has been reported that hemocytes play important roles in immunity, nutrient transportation, and growth hormone synthesis [38,39]. Furthermore, hemocytes are known to express spätzle proteins [40] and our results confirm this since we found the highest levels of TmSpz6 expression in hemocytes, suggesting that this tissue is important in T. molitor immune response. Taken together, these data suggest that TmSpz6 expression during transitional stages and in growth hormone-synthesizing tissues (hemocytes) under normal conditions is regulated by developmental hormones.
The active form of spätzle is generated during development [41] and/or the immune response to microbial infection [12,42]. Specifically, PGRP-SA or GNBP1 recognizes conserved bacterial or fungal molecules and activates the serine protease cascade that leads to the generation of mature spätzle [8,9]. The Toll receptor for the spätzle ligand is known to be located on the plasma membrane of fat body and hemocyte cells [43][44][45]. Therefore, to examine the induction of the TmSpz6-related immune response in T. molitor, larvae were challenged with E. coli, S. aureus, or C. albicans and then the expression of TmSpz6 was assessed in the main immune organs, such as hemocytes, fat body, and the gut. TmSpz6 was found to be highly induced at different time points following the injection of all tested microorganisms. Spätzle genes are activated upon microorganism infection as an effector of the Toll pathway. In M. sexta, spätzle-1 was upregulated at 24 h post-injection of E. coli or insoluble β-1,3-glucan [33]. In the current study, the highest TmSpz6 expression was observed in hemocytes against the three pathogens. The well-known gram-negative bacteria, E. coli possesses DAP-type PGN, which is recognized by PGRP-LC or -LE to activate the IMD pathway in Drosophila [46]. However, it is not surprising that a gram-negative bacterium (E. coli) induced the expression of TmSpz6 in current study, as it has already been reported that Tenebrio PGRP-SA can recognize the polymeric DAP-type peptidoglycan present in E. coli to activate the Toll receptor ligand spätzle in T. molitor [47].
The importance of TmSpz6 in the immune response against microbial infection was studied using RNAi. TmSpz6-silenced larvae showed significant susceptibility starting from 4th day of E. coli injection. This indicates that TmSpz6 plays a key role in the microbial defense response in T. molitor larvae. The expression of insect AMPs is mainly regulated by the evolutionarily conserved Toll and IMD pathways. Particularly, the spätzle-Toll-MyD88-Tube-Pell complexes and intracellular Dorsal and Dif binding to κB-related sequences play key roles in AMP production [12]. Spätzle plays a paramount role in activating Toll and is itself activated by other complexes [9]. Additionally, AMP gene expression was examined in TmSpz6-silenced larvae to investigate its function in the expression of AMP genes in response to microbial infection. The results reveal that TmSpz6 silencing suppressed the induction of several AMP gene expressions in response to microbial infection, supporting the survival study results. Most of the AMP genes that were suppressed when TmSpz6 was silenced encode AMPs that have activity against gram-negative bacteria, such as E. coli (Tene-2, Cec-2, Tene-4, and Cole-1) [24,[47][48][49][50], and gram-positive bacteria, such as S. aureus (Tene-3, Def-1, Def-2, Cec-2 and Tene-1) [51][52][53][54].

Conclusions
This study focused on the identification and immunological functional characterization of TmSpz6 in T. molitor. TmSpz6 is highly expressed in prepupal and 3-day-old pupal stages. In the tissue specific expression study, TmSpz6 was highly expressed in the hemocytes of late larvae. The induction patterns in response to microbial challenges revealed that TmSpz6 was highly upregulated in hemocytes at the 6 h-post injection of E. coli, S. aureus, and C. albicans. The survivability of TmSpz6-silenced larvae significantly decreased after the injection of E. coli or S. aureus. The loss of function of TmSpz6 significantly reduced the induction of various AMPs, particularly TmTen-2 and -3 in response to E. coli and S. aureus infection. Taken together, these results suggest that TmSpz6 plays an important role in regulating AMP expression and increases the survival of T. molitor against E. coli and S. aureus.

Conflicts of Interest:
The authors declare no conflict of interest.