1. Introduction
Pine wilt disease (PWD) is one of the most dangerous diseases in global forestry ecosystems, which is caused by the nematode
Bursaphelenchus xylophilus (pine wood nematode, PWN) [
1].
B. xylophilus develops from an egg to an adult through three propagative larval stages (the second-stage juveniles (J2), J3, and J4). The J1 stage molts to J2 within the egg. Under harsh conditions,
B. xylophilus molts from J2 to the third stage dispersal juvenile (D3), then to D4 in the presence of the vector beetle. The D4 nematodes are carried to new healthy host trees, completing their life cycle [
2]. It has resulted in devastating effects on the pine forests across Asia and Europe over the past century. Tree trunk injection with nematicides is a primary method for controlling PWD, leveraging the transpiration process of the trees to distribute the agents throughout affected areas [
3]. Abamectin [
4] and emamectin benzoate [
5] are commonly used for this purpose, targeting the GABA receptor and glutamate-gated chloride channels (GluCl) in invertebrates to paralyze nematodes [
6]. The repeated use of these nematicides can create selection pressure, increasing the risk of developing drug-resistant strains of PWN [
7,
8]. There is a pressing need to develop new nematicides and replace current treatments to manage PWD more effectively.
Succinate dehydrogenase inhibitors (SDHIs) represent a rapidly evolving class of pesticides targeting SDH. Possessing spectral inhibitory properties, SDHIs are extensively employed for fungal [
9,
10], acarid [
11], and nematode [
12] control. SDH comprises a transmembrane assembly composed of four protein subunits (SDHA to D), a flavin adenine dinucleotide (FAD) cofactor (associated with SDHA), three iron–sulfur clusters (housed within SDHB), and a heme moiety (positioned between SDHC and D). SDHA (flavin protein, FP) and SDHB (iron sulfide protein, IP) constitute the soluble components of complex II, exhibiting succinate dehydrogenase function. In contrast, SDHC and SDHD are membrane-integrated proteins pivotal for immobilizing FP and IP within the inner mitochondrial membrane, governing ubiquinone reductase activity. Lipid-soluble redox-active quinones at the Q site expedite electron and proton transport across the respiratory membrane complexes. Succinate dehydrogenase inhibitors bind to the ubiquinone pocket (Q site) within SDH (comprising SDHB, SDHC, and SDHD subunits), thereby impeding respiration via competitive antagonism [
9,
13]. This inhibition disrupts the conversion of succinate to fumarate and the reduction of ubiquinone to panthenol. Notably, the crystal structure of SDH has been elucidated in Escherichia coli, chickens, and pigs [
9].
Cyclobutrifluram, a novel SDHI nematicide developed by Syngenta, features a unique carboxamide structure with a four-membered ring, offering a new approach to nematicide development [
14]. To date, limited research has been conducted on the effectiveness of cyclobutrifluram. A study on
Caenorhabditis elegans indicated a significant reduction in germ cell quantity, pointing to potential impacts on survival and fertility [
15]. This nematicide operates by impeding the mitochondrial SDH complex, similar to the mechanism of fluopyram, a well-studied nematicide effective against
B. xylophilus [
16,
17]. With its analogous mechanism, cyclobutrifluram is anticipated to exhibit effectiveness in combating
B. xylophilus. Therefore, our objectives were as follows: (a) To assess the toxicity of cyclobutrifluram against
B. xylophilus, along with abamectin, emamectin benzoate, and fluopyram; (b) To investigate the effects of these agents on the reproduction, growth, and development of
B. xylophilus; (c) To evaluate the efficacy of cyclobutrifluram in controlling PWD in greenhouse and field settings; (d) To characterize four
sdh genes and their functions in
B. xylophilus; (e) To confirm that cyclobutrifluram targets the SDHs in
B. xylophilus. This study offers significant insights into the nematocidal activity of cyclobutrifluram against
B. xylophilus, providing a good basis for the development of new drugs against
B. xylophilus and for understanding the principle of control targeting SDH.
3. Discussion
Cyclobutrifluram, developed by Syngenta, is a novel SDHI that has demonstrated significant activity against pathogens but has not yet been registered for controlling plant-parasitic nematodes. This study marks the first utilization of cyclobutrifluram as an alternative agent against B. xylophilus, providing a theoretical foundation for the sustainable and effective control of PWD.
Before implementing trunk injection as a preventive measure against PWD, it is crucial to ascertain the nematocidal activity of the substance in question. Compared with the other three agents (emamectin benzoate, abamectin, fluopyram), cyclobutrifluram had the best nematocidal activity against
B. xylophilus, with an LC
50 value of 0.1078 mg·L
−1. In addition, cyclobutrifluram had a strong inhibitory effect on the fecundity. The female egg-laying rate decreased after being treated with this compound. These findings are consistent with those on
C. elegans, in which the number of progenies reduced from 247 ± 70 to 144 ± 95 [
15]. Moreover, half of the
B. xylophilus J2 in the cyclobutrifluram-treated group failed to reach J4, which may be because the development of nematodes was either slowed or stopped in a hypometabolic condition of chemical stress [
18]. It is similar to how sodium azide inhibits
C. elegans, which inhibits cytochrome C in the electron transport chain and causes cell cycle arrest and, eventually, larval arrest [
19]. Moreover, cyclobutrifluram significantly decreased the body lengths of both male and female first-generation nematodes. Several studies have shown that body lengths in
C. elegans requires a highly conserved signal transduction pathway (cGMP-EGL-4) regulated by a member of the TGFβ family, DBL-1 [
20]. We speculate that chemical signal affects the expression level of some guanylyl cyclase (GC), which, partnered with EGL-4, exerts effects on downstream functions. Moreover, cyclobutrifluram affects the reproductive system of nematodes, leading to a reduction in the number of germ cells [
15], which may indirectly lead to a reduction in average body length.
Cyclobutrifluram showed excellent preventive effects on PWD in both the greenhouse and the field. Pine trees infested with drug-treated nematodes displayed initial signs of wilting on the 40th day of inoculation, with all trees exhibiting wilting symptoms by the 90th day. The disease manifested itself one month later than in the control group. And, at a higher concentration of 20 mg·cm
−1 DBH, none of the treated trees died after a period of 24 months. Similarly, none of the EB-treated trees died after a period of 26 months, contrasting with a 33% mortality of non-treated pines [
5]. EB was used to control
B. xylophilus through GABA receptor and glutamate-gated chloride channels. Cyclobutrifluram in the present study was used to kill
B. xylophilus by SDHI. Post-treatment, the nematodes were suppressed through the drug’s specific mechanism, leading to a reduction in the nematode population and alleviation of the disease.
In this study, we characterized
sdha to
d four genes expressed in
B. xylophilus. After
sdhs-dsRNA treatment, the egg hatching rate, locomotor capacity, and body lengths of nematodes were significantly reduced, which is similar to reported RNAi phenotypes and mutations in electron transport chain molecules of
C. elegans [
21]. These observed characteristics suggest a compromised mitochondrial function, leading to adverse effects on the nematodes’ development and behavior. This mechanism of action is perhaps what makes cyclobutrifluram so effective. RNA interference techniques are widely used to identify pesticide target genes. The sensitivity of nematodes to succinate dehydrogenase inhibitory agents has been demonstrated [
22]. A resistance screen conducted on
C. elegans revealed that specific amino acid mutations within the SDHB, SDHC, and SDHD protein subunits of complex II conferred insensitivity to the wact-11-family compound. The wact-11 family shares a core structure that is closely related to fluopyram and cyclobutrifluram [
22,
23]. In the current study, RNAi of
sdhb/
c/
d greatly decreased cyclobutrifluram-induced mortality in
B. xylophilus, indicating the agent’s target within the SDH complex of the mitochondrial respiratory chain. Notably, the
sdhc-dsRNA treatment group exhibited significantly lower mortality rates compared to the other treatment groups. Molecular docking studies have further revealed that SDHC served as the primary target site for the agent on
B. xylophilus. SDHC mutants also show resistance to cyclobutrifluram and fluopimomide in
C. elegans [
12,
15]. SDHC mutants have a dysfunction of the SDH enzyme, leading to an abnormal energy metabolism with increased sensitivity to oxidative damage [
24]. These SDHC mutants eliminate the competition site between the drug and lipid-soluble redox-active quinones, thus rendering the nematodes drug-insensitive. These findings suggest that the primary mode of action of cyclobutrifluram against
B. xylophilus primarily involves its interaction with SDHC within the SDH enzyme complex.
In addition, Heydari et
al.‘s transcriptome enrichment analysis revealed that genes encoding cytochrome P450 and UDP glucosyltransferase (UGT) were highly expressed in
C. elegans when exposed to cyclobutrifluram [
15]. Since these genes play crucial roles in metabolism and detoxification, we hypothesize that
B. xylophilus may exhibit similar gene expression changes when exposed to cyclobutrifluram. Therefore, the next step of our study will focus specifically on the expression of these genes in
B. xylophilus. This will help us further elucidate the mechanism of action of cyclobutrifluram and aid in the development of more effective nematocidal strategies.
4. Materials and Methods
4.1. Nematodes
The
B. xylophilus specimens utilized in this study, labeled NXY61, were initially extracted from
Pinus massoniana trees infected in Zhejiang province, China. They were subsequently isolated and cultured on
Botrytis cinerea fungal mats, which were grown on 9 cm diameter potato dextrose agar (PDA) plates at 25 °C in darkness. The collection of nematodes at various synchronized stages (eggs, juveniles 2–4 (J2–J4), adults) was carried out using the methodology described by Zhou et al. [
25]. Unmated J4 female and male nematodes were separately cultured on
B. cinerea plates under the same conditions to obtain virgin adults after 24 h.
4.2. Chemicals
Technical grade abamectin and emamectin benzoate (95% concentration) were acquired from Zhejiang Shenghua Biok Biology Co., Ltd., Deqing, China. Fluopyram (96% concentration) was sourced from Bayer® CropScience (China) Co., Ltd., Hangzhou, China. Cyclobutrifluram (95% concentration) was supplied by Syngenta Biotechnology (China) Co., Ltd., Shanghai, China. The 5% emamectin benzoate micro-emulsion (ME) formulation consisted of 50 g·L−1 emamectin benzoate, 300 mL·L−1 n-butyl alcohol, 150 mL·L−1 octylphenol polyoxyethylene-10, and sterile distilled water. The 1.8% abamectin ME formulation comprised 18 g·L−1 abamectin, 30 mL·L−1 methanol, 150 mL·L−1 toluene, 80 mL·L−1 emulsifier OP-10, and sterile distilled water. The 5% fluopyram emulsifiable concentrate (EC) formulation included 50 g·L−1 fluopyram, 10 mL·L−1 emulsifier OP-10, and acetone. Cyclobutrifluram was formulated as a 5% EC in DMSO.
4.3. Toxicity Test against B. xylophilus
The toxicities of 5% ME emamectin benzoate, 1.8% ME abamectin, 5% EC fluopyram, and 5% EC cyclobutrifluram against
B. xylophilus were assessed using the dipping method [
26]. These agents were prepared in at least six mass concentration gradients (
Table S1), with one treatment for each concentration and distilled water serving as the control. Each well of a 96-well plate, pre-loaded with approximately 100 mixed-stage nematodes, received 100 μL of the pesticide solution. The plates were incubated at 25 °C, and after 24 h, the live and dead nematodes were counted. To avoid experimental errors, nematodes were washed and transferred to sterile water for 12 h. Nematodes were stimulated by shaking before counting. When nematodes were C- or L-shaped and not moving after stimulation with a fine needle, they were considered dead [
27]. This procedure was repeated three times for each treatment, with three replicates each time. Mortality rates were reported as percentage corrected mortality (±standard error), and the linear regression equation for toxicity was calculated using IBM SPSS Statistics 26. The LC
20, LC
50, and LC
90 values were then determined.
4.4. Effect of Four Nematicides on Reproduction
The four agents were prepared at sublethal LC
20 concentrations to assess their effects on reproduction. Ten virgin male and female adult nematodes were randomly selected and treated with 0.5 mL of the agents for 24 h, with distilled water serving as the control. They were then cleaned and placed on
B. cinerea plates, cultured at 25 °C in darkness. Reproduction was measured once the mycelia of
B. cinerea in any of the Petri dishes were exhausted, approximately after 8–9 days. Nematodes were extracted using the Baermann funnel technique [
28] and collected in a centrifuge tube, which was then filled to 10 mL with distilled water. The nematodes were killed with low heat before counting. A 100-μL well-mixed nematode suspension was drawn up with a pipette and placed on slides to count the numbers under a light microscope (Leica DMi1; Leica Microsystems, Wetzlar, Germany). The total volume was estimated after magnification by 100 times. This experiment was conducted three times, with three replicate plates per treatment.
4.5. Effect of Four Nematicides on Egg Deposition
The four agents were also prepared to assess their effects on female egg deposition. Ten pairs of virgin adult nematodes were extracted and randomly transferred to 3 cm Petri dishes with 2 mL of the agents at LC20 concentrations; distilled water served as the control. After mating and spawning, 36 h later, the number of eggs at the bottom of each Petri dish was counted using a light microscope. If an egg hatched into a J2 stage nematode, this count was included. The experiment was carried out three times, with three replicates per treatment. The number of eggs laid by each female in each replicate was calculated.
4.6. Effect of Four Nematicides on Egg Hatching Rate
To assess the effect of the four agents on egg hatching rate, eggs were collected from mixed-stage nematodes, which included a significant number of pregnant females, added to 3 cm Petri dishes. Approximately 100 eggs were laid in the dark for 1 h at 25 °C. The nematodes were then removed with a pipette, leaving only the eggs at the bottom of the dish. These eggs were treated with 2 mL of the agents at LC
20 concentrations, while distilled water was used for the control. At 36 h post-treatment, the number of hatched eggs (J2) in each treatment group was recorded using a light microscope. The egg-hatching rate was calculated as follows:
The experiment was performed three times, and each treatment was replicated three times.
4.7. Effect of Four Nematicides on Development Progress
The inhibitory effects of four agents at LC20 concentrations on the growth and development of B. xylophilus were analyzed, focusing on the proportion of sexually mature individuals as an indicator of nematode development. Synchronized J2 nematodes were treated with the four agents at LC20 concentrations for 24 h and washed and reared on B. cinerea in PDA culture plates, with distilled water as the control. The plates were incubated at 25 °C in darkness for 68 h, allowing the control group nematodes to reach sexual maturity. Nematodes were extracted and collected in a centrifuge tube. A 100-μL well-mixed nematode suspension containing approximately 100 nematodes was pipetted into 3 cm Petri dishes. The total number of nematodes and sexually mature individuals in each treatment group was observed and scored using a light microscope.
The sexual maturity rate was calculated using the following formula:
The experiment was performed three times, with three replicates per treatment.
4.8. Effect of Four Nematicides on Body Lengths of Offspring
To assess the effects of the four nematicides on offspring body lengths, assays were conducted with adult second-generation nematodes. Ten pairs of adult nematodes were treated with 0.5 mL of the agents for 24 h, then placed on B. cinerea mats for mating and egg laying, with distilled water added to the control. Their offspring were then extracted and collected in a centrifuge tube. Twenty sexually mature female and male adult nematodes were randomly selected, collected in a 1.5 mL centrifuge tube, and killed with low heat. A Nikon upright fluorescence microscope was used for photography, and ImageJ software (version 1.49) was used to measure body length. The experiment was repeated three times.
4.9. Control Efficacy of Cyclobutrifluram to B. xylophilus in the Greenhouse
The efficacy of cyclobutrifluram in inhibiting pathogenicity was tested. Three experimental groups were established. In the control group, suspensions containing 4000 nematodes were inoculated under the phloem of a 3-year-old black pine (
Pinus thunbergii Parl) tree. In the treatment group, nematodes were treated with cyclobutrifluram at LC
20 concentrations for 24 h before inoculation. Trees in the blank group were inoculated with distilled water. The inoculation site was the middle and upper parts of the trunk, with 10 replicates in each group. All trees were maintained in a greenhouse at 25 °C. The incidence of pine wilt was observed, and the pathogenicity of pine wood nematodes was analyzed. The infection rate of pine trees was used to assess
B. xylophilus infections during 100 days after infection [
29]. To check for the presence of
B. xylophilus in a tree 100 days after infection, 5 cm branches from the top, middle, and bottom were randomly sampled, cut up, and placed in a funnel. The presence of
B. xylophilus was observed with a microscope, and the number of nematodes per gram of branch was counted.
4.10. Preventative Effect against PWD under Field Conditions
The “infected area” was defined as a 20 m radius around the principally PWN-infected pine trees (
Figure 6a). To evaluate the preventative effect of cyclobutrifluram against PWD, healthy
P. massoniana (18–35 cm diameter at breast height) from the infected area were used in a test in a forest at Qianlang village, Shizhu Town, Yongkang City, Zhejiang Province (28°50′ N, 120°7′ E). For trunk injections, 2% cyclobutrifluram EC and 2% emamectin benzoate ME (as a positive control) were prepared. Cyclobutrifluram was tested at 0.5 and 1.0 mL·DBH
−1 volumes, while emamectin benzoate was tested at 1.0 mL·DBH
−1. In the blank control groups, no agents were injected. The treatments were randomly distributed in the infected area holes (8 mm diameter × 7–8 cm depth) and were drilled into the trunks of pine trees at a height of 1 m above ground (
Figure 6b). The appropriate dosages of each chemical treatment were injected into each hole using a pipette; this was performed on 10–15 June 2021, and only once. The preventative effect of each agent was determined by the mortality rate after 8, 16, and 24 months, with 41–152 trees used per treatment, and the experiment was repeated three times (
Table S2). A reddish–brown coloration of all needles represents tree death. All dead trees have been felled, and parts of their trunks chopped up to analyze for the presence of the
B. xylophilus.
4.11. Phylogenetic Analysis, Model Building, and Molecular Docking of SDHs
The amino acid sequence of the
B. xylophilus SDH subunits (SDHA: CAD5235524.1, SDHB: CAD5215503.1, SDHC: CAD5222053.1, SDHD: CAD5221188.1) were retrieved from NCBI. Phylogenetic analysis of the SDHs in
B. xylophilus with the amino acid sequences of this protein from other species was performed using MAGA software (version 11.0.10). A 3D structural model of
B. xylophilus SDHs was developed by homology modeling performed by the AlphaFold2 [
30]. The protein is a transmembrane complex comprising four protein subunits (SDHA to D). The experiment of SDH-autodocking with cyclobutrifluram was performed on
http://hdock.phys.hust.edu.cn/ (accessed on 3 February 2024) [
31].
4.12. Gene Clone of Four sdhs
B. xylophilus of developmental stages were collected, and their total RNAs were extracted. They were converted to cDNA for gene cloning and qPCR. Four
sdh genes (
sdha,
sdhb,
sdhc, and
sdhd) encode four nuclear-encoded subunits form the SDH complex in
B. xylophilus. Their cloning primers are designed (
Table S3) and cloned into a pGEM-T Easy vector (Promega, Madison, WI, USA). Four genes were cloned to generate dsRNA for RNAi.
4.13. The Relative Expression Levels of sdhs Analysed by RT-qPCR
Primers for the reference gene
β-actin (EU100952.1) and target genes of
B. xylophilus were used in qPCR to examine the expression levels (
Table S3). RT-qPCR was carried out using the qTOWER 2.2 qPCR System (Analytik JenaAG, Thuringia, Germany) with TB Green
® Premix Ex Taq II™ (TaKaRa, TliRNaseH Plus, Kusatsu, Japan). The relative
sdhs gene expression data were analyzed using the 2
−ΔΔCT.
4.14. dsRNA Synthesis and RNAi
T7 promoter sequences were added to the end of target genes’ cloning primers for the synthesis of dsRNA (
Table S3). The green fluorescent protein-encoding gene (
gfp, M62653.1) was used as the nonendogenous control. Four
sdh genes and GFP dsRNA fragments were synthesized using the MEGAscript
® T7 High Yield Transcription Kit (Thermo Fisher Scientific Inc., Waltham, MA, USA). Nematodes were soaked in RNAi solution for 24 h, which contained 4 μL of M9 buffer, 10 μg
sdha/b/c/d-dsRNA, and ddH
2O. Nematodes were soaked in M9 buffer without dsRNA as blank control. Nematodes were soaked with
gfp-dsRNA as exogenous control. All treatment solutions were up to 20 μL; each treatment had three replicates.
Virgin male and female nematodes were treated with different RNAi solutions for 24 h. For each group, 10 pairs of nematodes were selected for mixed culture, and the number of eggs laid by each female was counted after 36 h. After 24 h, ten hatched J2s were randomly selected from each group, and their motility was evaluated in terms of head swing frequency per minute. J2 was transferred to a B. cinerea mat and cultured into an adult. Ten male nematodes were selected, and their body lengths were measured. Each treatment had three replicates.
4.15. The Sensitivity of B. xylophilus to SDHs
The mixed-age B. xylophilus were cultured and collected, treated by sdh-dsRNA for 24 h in the treatment group, treated with gfp-dsRNA in the exogenous control group, and treated with ddH2O in the blank control group. The total RNA of mixed-age nematodes in each treatment group was extracted and reverse-transcribed into cDNA. The RNA interference efficiency of Bxy-sdh-dsRNA was detected by RT-qPCR. The other mixed-age nematodes in each treatment group were exposed to LC20, LC50, LC90 (0.031, 0.1078, 0.7211 mg/L) of cyclobutrifluram using the toxicity test method, as described above. Mortality was evaluated after treatment with cyclobutrifluram for 24 h. This experiment was conducted three times, with approximately 100 nematodes per treatment.
4.16. Data Analysis
All statistical analyses were conducted using Microsoft Excel 2019, and the data were expressed as mean ± standard error (SE). GraphPad Prism 8 was used for the homogeneity test of variance and one-way analysis of variance (ANOVA), and multiple comparisons were performed using Tukey’s (HSD) test (p = 0.05) to analyze the significant difference.