Molecular Regulation of Host Defense Responses Mediated by Biological Anti-TMV Agent Ningnanmycin

Ningnanmycin (NNM) belongs to microbial pesticides that display comprehensive antiviral activity against plant viruses. NNM treatment has been shown to efficiently delay or suppress the disease symptoms caused by tobacco mosaic virus (TMV) infection in local-inoculated or systemic-uninoculated tobacco leaves, respectively. However, the underlying molecular mechanism of NNM-mediated antiviral activity remains to be further elucidated. In this study, 414 differentially expressed genes (DEGs), including 383 which were up-regulated and 31 down-regulated, caused by NNM treatment in TMV-infected BY-2 protoplasts, were discovered by RNA-seq. In addition, KEGG analysis indicated significant enrichment of DEGs in the plant–pathogen interaction and MAPK signaling pathway. The up-regulated expression of crucial DEGs, including defense-responsive genes, such as the receptor-like kinase FLS2, RLK1, and the mitogen-activated protein kinase kinase kinase MAPKKK, calcium signaling genes, such as the calcium-binding protein CML19, as well as phytohormone responsive genes, such as the WRKY transcription factors WRKY40 and WRKY70, were confirmed by RT-qPCR. These findings provided valuable insights into the antiviral mechanisms of NNM, which indicated that the agent induces tobacco systemic resistance against TMV via activating multiple plant defense signaling pathways.


Introduction
Plant viruses infecting crops, vegetables, and ornamental plants significantly affect product quality and yields in agriculture [1]. Virus infection is a complicated process involving the molecular interaction between viruses and the hosts. Plants utilize multiple defense strategies against viruses, such as the inducement of innate pathogen-associated molecular pattern (PAMP)-triggered immunity (PTI) through immune receptor signaling to inhibit virus infection [2]. Furthermore, plants employ resistance proteins containing a nucleotide-binding leucine-rich repeat (NB-LRR) domain, which recognize viral proteins and subsequently activate effector-triggered immunity (ETI) and a hypersensitive response (HR) to restrict viruses in local necrotic spots from systemic infection [3]. In addition, the plant antiviral defense response is often accompanied by significant changes in phytohormone expression [4]. Studies also indicate that the induction of RNA silencing also significantly contribute to resistance in plants [5]. The tobacco mosaic virus (TMV) is one of the most serious plant viruses infecting multiple host species, which cause diseases in a wide variety of crops [6,7]. TMV belongs to the positive-strand RNA virus and encodes a 126 kDa and a 183 kDa protein that function as replicases, a 30 kDa movement protein (MP) that facilitates the movement of viruses between host cells, and a 17.5 kDa coat protein (CP) that plays an important role in virions formation [7]. In modern agriculture, green prevention strategies or agents for virus control are effective, environmentally friendly, but still under development. Plant virus inhibitors from metabolites of microbes have been considered as a potential alternative for chemical pesticides [8,9]. Streptomyces are major members of actinomycetes that have been reported to produce more than 30 secondary metabolites [10]. Ningnanmycin (NNM) is a microbial pesticide isolated from fermentation broth of Streptomyces noursei var. xichangensis and is characterized by resistance enhancement, high efficiency, and low toxicity in host plants. Studies have shown that NNM promotes the expression of pathogenesis-related proteins, PAL, POD, and SOD activity, enhances salicylic acid (SA) biosynthesis, and induces systemic resistance in the host plants [11][12][13]. Furthermore, NNM has been shown to inhibit the polymerization process of TMV-CP in vitro [14]. However, the precise antiviral mode of action, especially the host signaling pathway and defense responsive genes involved in the resistance against TMV induced by NNM, remains to be further elucidated. The high-throughput sequencing techniques (such as Illumina RNA-seq) provide a powerful tool to clarify the transcriptomic variations of the host plants in response to biological antiviral agents [15,16].
In this study, we show that NNM effectively suppresses the systemic infection of TMV in planta and significantly inhibits the viral RNA accumulation in BY-2 protoplasts. The results of transcriptome analysis and RT-qPCR indicate that various defense-responsive, immune signaling, calcium signaling, and phytohormone responsive genes are significantly up-or down-regulated by NNM treatment. This study provides a novel insight into the identification of crucial genes and pathways involved in resistance against virus infection in response to biological agents.

NNM Treatment on N. benthamiana and BY-2 Protoplasts Inoculated with TMV
The agent 8% NNM was purchased from Deqiang Biological Co. Ltd. (Haerbin, China). To prepare the virus inoculum, the plant virus of TMV Shenyang isolate was collected from the tobacco planted area in the Shenyang, Liaoning province of northwest China. The complete nucleotide sequence of TMV-SY was determined (no. MG516107) and used for the construction of an infectious clone of pCB-TMV-SY through homologuous recombination techniques [17]. TMV virions were extracted and purified from the pCB-TMV-SY-inoculated N. benthamiana leaves following Gooding's method [18], and adjusted to a concentration of 40 µg/mL with 10 mM PBS buffer. N. benthamiana plants at a leaf stage of six to seven, cultivated at the 25 • C climate-control chamber were used for NNM treatment and virus inoculations. The 400 µg/mL and 200 µg/mL concentration of NNM diluted by distilled water was sprayed onto N. benthamiana and infiltrated with Agrobacteriums (OD 600 = 0.2) containing pCB-TMV-SY and an empty vector. Moreover, plants with H 2 O treatment were inoculated by TMV, while healthy plants without NNM treatment and TMV inoculation were served as the mock. Three plants were used in each of the treatments (i.e., two concentrations of NNM treatment, H 2 O treatment, and the mock) as biological replicates, and three individual leaves of each plant were sampled and pooled for further study. RNA extracted from the TMV-inoculated (I) leaves and the upper (U) un-infiltrated leaves ( Figure 1A) were subjected to a northern blot to detect viral RNA accumulation after 7 days of incubation. The experiments were performed with three biological replicates for statistical analysis (p < 0.05). In the BY-2 protoplasts experiment, BY-2 suspension cells were incubated with cell wall hydrolase buffer (cellulose RS 10 mg/mL and Pectolyase Y23 1 mg/mL in 0.4 M Mannitol buffer) at 25 • C for 3 h ( Figure 1C). Virus inoculation in the protoplasts was performed using polyethylene glycol (PEG) solution (PEG 6000 4g, 0.5 mL H 2 O, 5 mL 0.8M mannitol, 1 mL 1 M Ca(NO 3 ) 2 ). BY-2 protoplasts inoculated by 0.1 mg of TMV virions were incubated with 400 µg/mL, 200 µg/mL, and 100 µg/mL NNM diluted in W1 buffer (0.5 M Mannitol,4 mM MES, and 20 mM KCl). The BY-2 protoplasts experiment were carried out with three biological replicates for statistical analysis (p < 0.05).

Identification of the Genes in Response to NNM by RNA-Seq
To define the mode of action for NNM leading to inhibition of TMV RNA accumulation, we used transcriptome analysis to clarify crucial genes in TMV-inoculated tobacco BY-2 protoplasts in response to NNM. There were 69,374,590 and 61,272,488 clean reads from NNM treatment and control libraries ( Table 1). The total DEGs in response to NNM were shown in Table S2, and annotation of the DEGs in KEGG pathways were shown in Table S3. The volcano plot analysis indicated the significantly up-and down-regulated DEGs between the NNM and control treatment group (Figure 2A). There were 414 genes differentially expressed (FDR < 0.05 and ≥2-fold change) between the NNM treatment and control treatment samples, including 383 up-regulated and 31 down-regulated DEGs ( Figure 2B) (Table S4). These crucial DEGs were classified into various functions, including catalytic activity, binding, as well as metabolic and cellular processing by GO analysis ( Figure 3A). In addition, a total of 46 DEGs were annotated to 19 different KEGG pathways (Table S5). The results indicated that plant-pathogen interaction is the most enriched category that

Northern Blot Analysis
Total RNA was extracted from NNM and mock treatment N. benthamiana leaves or BY-2 protoplasts inoculated by TMV with TRIzon Reagent (CWBIO, Beijing, China) according to the manufacturer's protocol. The extracted RNA of each treatment group was adjusted to 10 µg and subjected to northern blot analysis as described [19] using a DIG High Prime DNA Labeling and Detection Starter Kit II (Roche, Mannheim, Germany). The digoxigenin-labelled RNA probes for TMV positive-and negative-strand RNA have been previously described [20]. The RNA signals were detected with a chemical luminous imaging system, Tanon 5200 (Tanon, Shanghai, China).

RNA Extraction, cDNA Library Construction, and Illumina Sequencing
To clarify the crucial differentially expressed genes (DEGs) induced by NNM in the TMV-infected plant cells, total RNA was extracted from NNM and mock treatment BY-2 protoplasts at 20 hpi with a TRIzon Reagent (CWBIO, Beijing, China) according to the manufacturer's protocol. Equal quantities of 10 RNA samples per treatment group were mixed together for the RNA pool. The mRNA was purified by oligo-dT beads (Qiagen, Hilden, Germany) and fragmented into approximately 300 nt pieces. The reverse-transcribed cDNA fragments were purified and washed for end repair and ligated to sequencing adapters. The final cDNA library was constructed by PCR enrichment and sequenced through Hiseq X ten Illumina sequencing platforms by GENEWIZ Technology Co. Ltd. (Suzhou, China). The raw reads were submitted to the SRA database at NCBI with accession numbers SRR8690256 and SRR8568069. The read counts for each matched gene were normalized with RPKM (reads per kilo bases per million reads) to calculate its expression level. Significant differentially expressed genes (DEGs) between the NNM treatment and control treatment groups were shown in a volcano plot based on the significance false discovery rate (FDR) <0.05 and log2 fold change of >1.0 or <−1.0. In addition, all of the DEGs were subjected to the Gene Ontology (GO) analysis and mapped to the Kyoto Encyclopedia of Genes and Genomes (KEGG) pathway to clarify the main biological functions and pathways.

Real-Time Quantitative PCR
To validate the transcriptome results, RNA extracted from NNM and control treatment BY-2 protoplasts at 20 hpi was subjected to reverse transcription to generate cDNA using a FastKing RT Kit (TIANGEN, Beijing, China). RT-qPCR was performed using SYBR Premix Ex Taq II (TaKaRa, Dalian, China) according to the manufacturer's protocol, and the conditions were as follows: 5 min at 95 • C, followed by 40 cycles at 95 • C for 30 s, 55 • C for 30 s, and 72 • C for 40 s. The relative gene expressions were analyzed by ABI StepOne Plus (Applied biosystems, Foster City, CA, USA) and calculated by the 2 -∆∆CT method using actin as a reference gene with three independent biological replicates. The primers used in RT-qPCR are listed in Table S1.

NNM Treatment-Inhibited TMV Systemic Infection in Planta and Viral Accumulation in Protoplasts
N. benthamiana plants were used to verify the anti-viral effect of NNM on the RNA accumulation and systemic infection of TMV in planta ( Figure 1A). The results showed that 400 µg/mL and 200 µg/mL NNM treatment on TMV = inoculated (I) leaves exhibited delays in discoloration or mosaic symptoms. In addition, the upper (U) un-inoculated leaves of the NNM-treated plants did not display any viral disease symptoms at 7 days post-inoculation (dpi) [21]. Furthermore, NNM effectively and reproducibly reduced accumulation of viral RNA in the inoculated and upper leaves of N. benthamiana in the biological replicates at 7 dpi ( Figure 1B), which indicated that NNM treatment suppressed and delayed the systemic infection of TMV.
Efficient long-distance movement and systemic infection of plant viruses require rapid replication of the viral genome in single cells. Therefore, tobacco BY-2 cells were used to test the effect of NNM on TMV viral accumulation in single plant protoplasts ( Figure 1C). The results demonstrated that the accumulation of genome RNA, especially the negative strand RNA of TMV in BY-2 protoplasts at 20 hpi, was progressively inhibited with increased concentration of NNM from 100 to 400 µg/mL ( Figure 1D). When the concentration of NNM was lower than 50 µg/mL, the antiviral effect of NNM on TMV in BY-2 protoplasts was extremely low [21]. To exclude the possibility that NNM may affect Agrobacterium infection in the plants, we treated Nicotiana benthamiana with 200 µg/mL, 400 µg/mL NNM, and distilled water 1 day after transient expression of green fluorescent protein (GFP) through agro-infiltration using pGD-GFP, and observed the GFP fluorescence 1 to 2 days after the agent treatment. The repeated results indicated that NNM treatment did not affect the GFP expression [21], which suggested that the agent has no obvious impact on Agrobacterium infection or gene expression. Taken together, the results indicate that NNM inhibits the systemic infection of TMV in planta and the viral accumulation in the single cells.

Identification of the Genes in Response to NNM by RNA-Seq
To define the mode of action for NNM leading to inhibition of TMV RNA accumulation, we used transcriptome analysis to clarify crucial genes in TMV-inoculated tobacco BY-2 protoplasts in response to NNM. There were 69,374,590 and 61,272,488 clean reads from NNM treatment and control libraries ( Table 1). The total DEGs in response to NNM were shown in Table S2, and annotation of the DEGs in KEGG pathways were shown in Table S3. The volcano plot analysis indicated the significantly up-and down-regulated DEGs between the NNM and control treatment group (Figure 2A). There were 414 genes differentially expressed (FDR < 0.05 and ≥2-fold change) between the NNM treatment and control treatment samples, including 383 up-regulated and 31 down-regulated DEGs ( Figure 2B) (Table S4). These crucial DEGs were classified into various functions, including catalytic activity, binding, as well as metabolic and cellular processing by GO analysis ( Figure 3A). In addition, a total of 46 DEGs were annotated to 19 different KEGG pathways (Table S5). The results indicated that plant-pathogen interaction is the most enriched category that shows significantly differential expression in KEGG analysis ( Figure 3B), especially in the pathway of PAMP-triggered immunity ( Figure S1) and MAPK signaling ( Figure S2). shows significantly differential expression in KEGG analysis ( Figure 3B), especially in the pathway of PAMP-triggered immunity ( Figure S1) and MAPK signaling ( Figure S2).  An equal volume of sterile water treatment was used as a control. * indicate a significant difference (p < 0.05) and ** indicate a significant difference (p < 0.01).

Plant Immunity, Metal Ion, and Phytohormone Signaling Response Induced by NNM
In this study, results of RNA-seq indicated that NNM treatment can induce plant immunity through regulating gene expression, such as receptor-like kinases (RLKs), PRRs, and other genes involved in the defense response and host-pathogen interaction ( Table 2). The metal ion, especially Ca 2+ , is also considered to be a critical component of immune-signaling pathways [22]. Here, our results indicated that many lines of genes involved in calcium signaling were significantly upregulated by NNM, such as the calmodulin-like protein 19 (CML19), CML41, CML45, and various genes involved in the binding, uptake, and transportation of calcium (Table 3). Plant virus infections and host resistance responses were frequently accompanied by phytohormone alterations [3,23]. In particular, phytohormone-responsive genes, such as the WRKY transcription factors WRKY40 and WRKY70, as well as ethylene, auxin, and abscisic acid (ABA)-responsive genes and/or transcription factors were differentially regulated by NNM (Table 4).

Plant Immunity, Metal Ion, and Phytohormone Signaling Response Induced by NNM
In this study, results of RNA-seq indicated that NNM treatment can induce plant immunity through regulating gene expression, such as receptor-like kinases (RLKs), PRRs, and other genes involved in the defense response and host-pathogen interaction ( Table 2). The metal ion, especially Ca 2+ , is also considered to be a critical component of immune-signaling pathways [22]. Here, our results indicated that many lines of genes involved in calcium signaling were significantly up-regulated by NNM, such as the calmodulin-like protein 19 (CML19), CML41, CML45, and various genes involved in the binding, uptake, and transportation of calcium (Table 3). Plant virus infections and host resistance responses were frequently accompanied by phytohormone alterations [3,23]. In particular, phytohormone-responsive genes, such as the WRKY transcription factors WRKY40 and WRKY70, as well as ethylene, auxin, and abscisic acid (ABA)-responsive genes and/or transcription factors were differentially regulated by NNM (Table 4).

Verification of DEGs by Real-Time Quantitative PCR
In order to reveal the regulation of NNM treatment on host gene expression and its antiviral effect, nine crucial DEGs corresponding with resistance, immunity signaling, calcium signaling, and phytohormone response were selected for RT-qPCR verification. The selected genes for comparison included the receptor-like kinase FLS2 (LOC107827601), S-receptor-like serine/threonine-protein kinase RLK1 (LOC107816125), mitogen-activated YODA-like protein kinase kinase kinase (MAPKKK, LOC107821703), WRKY40 (LOC107792337), WRKY70 (LOC107782765), RNA-dependent 1-like RNA polymerase (RDR1, LOC107827981), putative calcium-binding protein CML19 (LOC107808229), putative zinc finger protein ZAT12 (LOC107806768), and regulatory protein non-expressor pathogenesis-related genes 1 (NPR1) (LOC107831756). The results of RT-qPCR showed that the nine DEGs which were selected were significantly up-regulated by NNM, which were consistent with the results of RNA-seq ( Figure 2C).

Discussion
Plant viruses are an obligate parasite, which cannot replicate their genomes or move from cell to cell without the assistance of host factors. therefore, virus-host interactions played crucial roles in the multiplication and systemic infection of various plant viruses [65]. The effective plant antiviral agents can inhibit viruses by directly targeting viral nucleic acids or proteins, or indirectly control viruses by regulating the host responses, such as phytohormone expression and various signaling pathways to affect the balance of the virus-host interaction [3]. NNM plays multiple functions and roles by the direct impact on viruses and the induction of the host defense, respectively. For example, a study indicated that NNM can interact with TMV-CP and inhibit the polymerization of TMV virions [14]. On the other hand, a comparative analysis of RNA-seq of tobacco leaves under NNM-treated and non-treated ones was performed, in which the defense-related genes were induced by NNM and identified to contribute the plant response to CMV infection [13]. Therefore, it is possible that NNM Viruses 2019, 11, 815 9 of 14 has potential roles by regulating host defense-regulated responses and directly affecting the TMV assembly. In the present study, we used the RNA-seq and RT-qPCR to elucidate more crucial genes associated with host-resistance responses by NNM regulation against TMV. A model of the possible induced effects and regulation of the crucial DEGs and signaling pathways involved in TMV resistance are shown in Figure 4. indicated that NNM can interact with TMV-CP and inhibit the polymerization of TMV virions [14]. On the other hand, a comparative analysis of RNA-seq of tobacco leaves under NNM-treated and non-treated ones was performed, in which the defense-related genes were induced by NNM and identified to contribute the plant response to CMV infection [13]. Therefore, it is possible that NNM has potential roles by regulating host defense-regulated responses and directly affecting the TMV assembly. In the present study, we used the RNA-seq and RT-qPCR to elucidate more crucial genes associated with host-resistance responses by NNM regulation against TMV. A model of the possible induced effects and regulation of the crucial DEGs and signaling pathways involved in TMV resistance are shown in Figure 4. The tobacco BY-2 suspension cultured cell has been well-applied in the subject of plant physiology and pathology. The BY-2 protoplast is proved to be an effective system for agents screening and clarification of their mode of action. For example, BY-2 cells were treated with microbial-derived metabolite from Cladosporium herbarum, which results in significant up-regulation of host defense-related genes [66]. In this study, our results showed that NNM treatment effectively inhibited viral RNA accumulation of TMV and significantly regulated many lines of potential virus resistance genes in the tobacco BY-2 protoplasts.
Application of biological agents is a very effective and environmentally safe strategy to control viruses by inducing host defense responses [67]. PTI is an important defense response induced by perception of viral PAMPs by pattern recognition receptors (PRRs) [2]. FLAGELLIN-SENSING2 (FLS2) and RLK1 are well-conserved PRRs, being critical for the perception of conserved microbeassociated molecular patterns (MAMPs) to activate PTI in different plant species [37,38]. After recognition of invading pathogens by PRRs, mitogen-activated protein kinases (MAPKs) cascades are rapidly activated, and the transduction signal can eventually activate various WRKY transcription factors in plants [2]. Notably, many studies have shown that WRKY transcription factors from various plant species are induced in response to viral infection [68,69]. In this study, our results showed that NMM induced a significant up-regulation of FLS2, RLK1, MAPKKK, WRKY40, and WRKY70, which indicated that NNM can effectively inhibit TMV, possibly through positively regulating the PTI pathway. Induction of ZAT12 is indicated to be closely related with the oxidative stress response, and serves as an abiotic stress marker [43]. Our previous work has shown that the The tobacco BY-2 suspension cultured cell has been well-applied in the subject of plant physiology and pathology. The BY-2 protoplast is proved to be an effective system for agents screening and clarification of their mode of action. For example, BY-2 cells were treated with microbial-derived metabolite from Cladosporium herbarum, which results in significant up-regulation of host defense-related genes [66]. In this study, our results showed that NNM treatment effectively inhibited viral RNA accumulation of TMV and significantly regulated many lines of potential virus resistance genes in the tobacco BY-2 protoplasts.
Application of biological agents is a very effective and environmentally safe strategy to control viruses by inducing host defense responses [67]. PTI is an important defense response induced by perception of viral PAMPs by pattern recognition receptors (PRRs) [2]. FLAGELLIN-SENSING2 (FLS2) and RLK1 are well-conserved PRRs, being critical for the perception of conserved microbe-associated molecular patterns (MAMPs) to activate PTI in different plant species [37,38]. After recognition of invading pathogens by PRRs, mitogen-activated protein kinases (MAPKs) cascades are rapidly activated, and the transduction signal can eventually activate various WRKY transcription factors in plants [2]. Notably, many studies have shown that WRKY transcription factors from various plant species are induced in response to viral infection [68,69]. In this study, our results showed that NMM induced a significant up-regulation of FLS2, RLK1, MAPKKK, WRKY40, and WRKY70, which indicated that NNM can effectively inhibit TMV, possibly through positively regulating the PTI pathway. Induction of ZAT12 is indicated to be closely related with the oxidative stress response, and serves as an abiotic stress marker [43]. Our previous work has shown that the biological agent of cytosinpeptidemycin significantly induced up-regulation of ZAT12 [20]. In this work, gene expression of ZAT12 was significantly up-regulated under NNM treatment. However, the potential functions of ZAT12 involved in the anti-virus mechanism still remains to be clarified. In addition, various receptor-like kinases, as well as defense-and stress-responsive genes (Table 2) were differentially regulated by NNM, and their possible roles involved in virus resistance still need to be further investigated.
Calcium is an essential element needed for the growth and development of plants [70]. Ca 2+ is a secondary messenger involved in diverse crucial signaling pathways in plants through signals of abiotic and biotic stimuli [71]. The calmodulin-like protein CML19 is possibly involved in drought response [59], and the CML46 and CML47 have been reported to negatively regulate SA [58]. Ca 2+ signaling is also a critical component of plant immune response [71]. The perception of pathogen attacks induces an influx of Ca 2+ into the cytosol, which is decoded into downstream responses ultimately leading to defense. For example, the Calmodulin-like protein CML41 localizes at plasmodesmata and induces plasmodesmal closure during bacterial immune responses [72]. In this study, our results showed that a variety of genes involved in calcium signaling were significantly induced by NNM (Table 3). These results indicate that calcium signaling can play vital roles in NNM-mediated resistance to TMV.
Plants can use elaborate strategies by inducing phytohormone-signaling networks to get through abiotic or biotic stresses, as well as inducing resistance response to pathogen infection [3,23]. Our results demonstrated that various phytohormone-responsive genes, including WRKY transcription factors, ethylene, auxin, and ABA-responsive genes or transcription factors were differentially regulated by NNM (Table 4). WRKY40 mainly functions as a central negative regulator of the expression of ABA-responsive genes [29]. In addition, WRKY40 was also reported to associate with a transcription factor BZR1 to mediate plant immune signaling [73]. WRKY70 is an important node of convergence between SA and JA signaling in Arabidopsis [74]. Overexpression of WRKY70 can enhance the expression of SA-responsive PR genes and negatively affects transcription of JA-responsive genes [27,74]. In addition, NNM induced up-regulation of NPR1 ( Figure 2C) that regulates SA and systemic acquired resistance (SAR), which is consistent with the results of a previous study [11]. Such results indicated that NNM induced biosynthesis of SA, that may contribute to virus resistance. Ethylene responsive factors (ERFs) play vital roles in plant pathogen defense responses. A typical transcription factor, ERF109 belongs to the stress responsive genes, and was reported to improve salt tolerance and delay PCD in plants [63]. In the present study, ERF109 was significantly up-regulated by NNM, which suggests the possible involvement of ERF109 in virus defense.
RNA silencing (or RNAi) is an effective defense mechanism against viruses, with remarkable specificity and adaptability [75,76]. Host proteins, such as the DICER-LIKE proteins (DCLs), Argonaute (AGO) proteins, and RNA-dependent RNA polymerase (RDR) proteins, are core components of plant RNA silencing pathways against plant viruses [75,76]. Studies have indicated that the RdR1 induces the basal defense response [31,32], and also regulates RNA silencing-related gene expression to suppress the replication and movement of TMV [32]. In addition, the tobacco calmodulin-like protein was reported to promote RNA silencing by binding to and directing degradation of the virus RNA silencing suppressors [77,78]. Taken together, the remarkable up-regulation of RdR1 and CMLs induced by NNM possibly promoted RNA silencing to suppress virus infection, which provides a new perspective for the development of novel antiviral agents.
In summary, the effect and mode of actions of NNM on TMV through induction of host resistance were explored. We identified various crucial genes involved in host stress responses, signaling transduction, and various phytohormone responses by NNM treatment (Figure 4). We further hypothesized that NNM possibly regulates RNA silencing in controlling the virus. This work provided a novel insight into the antiviral mode of action for the biological agent of NNM, and also provided a theoretical basis for the development of highly specific and effective antiviral agents.