Characterization of Migration and Induced Resistance of Rhizobium Vitis Strain ARK-1, a Biological Control Agent Against Grapevine Crown Gall Disease

A nonpathogenic strain ARK-1 of Rhizobium vitis has an antagonistic activity toward tumorigenic (Ti) strain of R. vitis, a causal agent of grapevine crown gall disease, and works as a biocontrol agent. We have demonstrated that the gall formation was fully suppressed when ARK-1 was co-inoculated with Ti into the grapevine stem at a 1:1 ratio. For practical use of ARK-1 in agriculture, understanding the temporal dynamics of the bacterial habitat on host plants and the biocontrol property are needed in order to develop proper application methods. Here we demonstrated that the gall incidence by Ti was reduced to about 50% when ARK-1 was pre-inoculated at both upper and lower positions on the grapevine stem 3 cm away from the Ti-inoculation point 5 days before. The bacterial cell detection assay in the grapevine tissue revealed that ARK-1 could migrate at least 3 cm in 5 days. Inoculations of ARK-1 or Ti induced expression of marker genes for defense-related phytohormones such as salicylic acid, jasmonic acid, and ethylene in grapevine within 3 days but they were diminished by 6 days. Inoculation of Ti 5 days after ARK-1 pre-inoculation induced expression of the marker genes except for the LOX-9 gene in a basically similar way to those without the pre-inoculation, suggesting that ARK-1 did not induce typical acquired systemic resistance or induced systemic resistance in grapevine, while the transcript of LOX-9 was detected at 24 and 48 hours after the Ti inoculation when ARK-1 was pre-inoculated, unlike the un-inoculated condition. ARK-1 primed the induction of certain defense genes and it may take part in its biocontrol activity. were collected at the indicated time points. The relative rates of defense-related genes PR-1 (A), PR-4 (B), LOX-9 (C), PDF1.2 (D), and ERF (E) were measured using reverse transcriptase quantitative polymerase chain reaction (RT-qPCR) with specic primers. Data are means ±SEM of relative expression rates to each value with water at 12 hours post-inoculation (hpi), which had a value of 1.0 (n = 3). Different letters represent signicant differences according to Tukey’s HSD (P ≤ 0.05). The experiments were repeated 3 times with similar results. inoculated into both upper and lower positions in seedlings, and Ti was inoculated into the middle position after 5 days. Tissues 5 mm away from the inoculation sites were collected at the indicated time points. The relative expressions of defense-related genes PR-1 (A), PR-4 (B), LOX-9 (C), PDF1.2 (D), and ERF (E) were measured using reverse transcriptase quantitative polymerase chain reaction (RT-qPCR) with specic primers. Data are means ±SEM of relative expression rates to each value with water at 12 hours post-inoculation (hpi), which had a value of 1.0 (n = 3). Different letters represent signicant differences according to Tukey’s HSD (P ≤ 0.05). The experiments were repeated 3 times with similar results.


Introduction
Grapevine (Vitis vinifera L.) crown gall is caused mainly by Rhizobium vitis (Ti) [syn. Agrobacterium vitis (Ti), A. tumefaciens biovar 3], where "Ti" means "tumor-inducing" or "tumorigenic." In this paper, we follow the nomenclature for Rhizobium species adopted by Young et al. 1 to avoid confusion. This pathogen enters the grapevine through wounds due to a variety of causes, such as winter injury, mechanical damage, and grafting 2 . R. vitis (Ti) causes crown gall by transferring the T-DNA region of the tumor-inducing bacterial plasmid (Ti-plasmid) to the host cell, which subsequently integrates into the plant host genome [3][4][5] . The inserted T-DNA contains genes for biosynthesis of plant growth hormones, which induce hyperplastic and hypertrophic cell proliferation that results in galls [6][7] . Invasion of vascular tissue by galls can result in vine death [8][9] .
The history of the search for viable biological control agents for crown gall goes back to the early 1970s 10 . Among potential biological agents against crown gall, two have been extensively studied. Rhizobium rhizogenes (=A. rhizogenes, A. radiobacter biovar 2) strain K84 has been used since the early 1970s. It inhibits the growth of some Rhizobium species and reduces crown gall [10][11][12] . K84 produces an antimicrobial molecule, agrocin 84, that is antagonistic to particular strains of Rhizobium [13][14] . K84 is used today for the prevention of crown gall predominantly in stone fruit and apple but also other fruit and nut trees. However, K84 is ineffective against crown gall disease in grapevine caused by R. vitis 7,[15][16] .
Although several laboratories have attempted to develop biological measures to control grapevine crown gall, there are no successful agents to control this disease, especially under eld conditions [17][18][19][20] .
Moreover, we identi ed a nonpathogenic R. vitis strain ARK-1 as a new antagonistic strain 16 . ARK-1 neither carries the Ti-plasmid nor causes disease symptoms 16 . ARK-1 is endophytic in grapevine and induces no necrosis in the host plant. It provided better control against grapevine crown gall than VAR03-1 in eld trials 25 . ARK-1 is also effective at controlling crown gall in other plant species such as tomato, pear, peach, apple, and rose 26 . Suppression of gall formation by ARK-1 was observed when it was coinoculated with Ti into a grapevine stem. The culture ltrate (CF) of ARK-1 (without cells) or heat-killed culture was not able to inhibit tumor formation on grapevine 16 . These results indicate that ARK-1 must be alive to effectively antagonize gall formation by Ti 27 . ARK-1 has antibiotic activity against Ti strains of Rhizobium spp. and this direct antagonism would be an important mechanism for its biocontrol activity 28 .
Pre-treatment of grapevine roots with ARK-1 cell suspension before planting in Ti-contaminated soil also effectively suppressed gall formation in roots 16,25 . ARK-1 slowed down the population growth of Ti at inoculation sites 28,29 and suppressed the expression of virulence (vir) genes (virA, virD2, virD3, virE2, and virG on Ti-plasmid) that are required for plant cell transformation by T-DNA 29,30 . To develop a practical application method of ARK-1 in agriculture, an understanding of colonization dynamics on host plants is required. It is known that Ti strains can move inside grapevines through the vascular system and spread widely, thereby developing galls not only on roots but also shoots 7, 31-32 . ARK-1 is also expected to migrate through grapevine tissues but it has not yet been characterized.
Plants protect themselves from microorganisms by inducing a coordinated defense system triggered by immunity-related phytohormones such as salicylic acid (SA), jasmonic acid (JA), and ethylene (ET) 33 . To counteract biotrophic pathogens, the SA-dependent signaling pathway plays an important role. In contrast, plants induce defenses against necrotrophic pathogens, insect herbivores, and wounding using JA and ET. In both cases, whole plant tissues become sensitive after an initial attack and respond quickly and strongly to secondary challenges to confer a broad-spectrum resistance. These phenomena are known as systemic acquired resistance (SAR) and wound-induced systemic resistance (WSR), respectively [34][35][36] . Fluorescent pseudomonads, which are known as plant growth-promoting rhizobacteria (PGPR), enhance plant immunity in above-ground parts by a mechanism called induced systemic resistance (ISR) 37 , and this is dependent on JA and ET but not SA 38 . Interestingly, ARK-1 also suppressed tumor formation in grapevine shoots when it was co-inoculated with a Ti strain whose growth was not inhibited by ARK-1 in the antibiosis assay 28 . Based on this result, we expect that ARK-1 has another mechanism other than antibiosis, such as immune priming or con ict of habitat, for the suppression of crown gall. However, it remains unclear.
In this study, we veri ed that ARK-1 can move along the grapevine stem and suppress gall formation by Ti at places distant from the inoculation site. ARK-1 reached positions 3 cm away within 5 days and reduced disease incidence by Ti to about 50% at that position. The inoculation of ARK-1 upregulated defense-related genes 24-72 hours post-inoculation (hpi) in the same manner as Ti in grapevine, but the upregulation was transient. Pre-inoculation of ARK-1 did not enhance expression of the defense-related genes tested upon Ti inoculation except for LOX-9, suggesting the possibility of an atypical priming effect of ARK-1 on particular genes.

Bacterial strains
The bacterial strains used in this study are listed in Table S1. Potato sucrose agar (PSA) medium was used for culture of the bacteria. A streptomycin (St)-and copper sulfate (CuSO 4 )-resistant ARK-1 mutant (ARK-1sc) was selected using PSA medium containing 500 μg/mL St and 250 μg/mL CuSO 4 25 . A nalidixic acid (nal)-resistant VAT03-9 (Ti) mutant (VAT03-9n) was obtained using PSA medium supplemented with 50 μg/mL nal 29 . The growth rates of these mutants in PSA medium were comparable to that of the wild-type 29 .
Gall inhibition assay in grapevine seedlings Grapevine seedlings (Vitis vinifera cv. 'Neo Muscat') were grown from seed. One-year-old grapevine shoots were inoculated using previously established methods (Kawaguchi et al. 2005(Kawaguchi et al. , 2007. In this study, four inoculation patterns (treatments) with three different inoculation points were used (Table 1, Fig. S1). Each grapevine seedling (at one plant per pot) had three inoculation sites (upper, middle, and lower) with approximately 3.0 cm spacing. In treatment (i), Ti was inoculated into the middle point, and at the same time sterile distilled water was inoculated into the upper and lower points. In treatment (ii), Ti was inoculated into the middle point, and at the same time ARK-1 was inoculated into the upper and lower points. In treatment (iii), sterile distilled water was pre-inoculated into the upper and lower points, and 5 days later, Ti was inoculated into the middle point. In treatment (iv), ARK-1 was preinoculated into the upper and lower points and, inoculated into the middle point after 5 days. Ten plants were used for each treatment. The experiments were performed independently 3 times. Grapevine seedlings were grown in a greenhouse at 20-35°C with natural sunlight (photoperiod: 12 to 14 h light: 10 to 12 h dark). The inoculated seedlings were kept in the same environment for 5 months, and gall formation rates and gall sizes (diameter) (mm) (the widest point measured with a digital caliper) were recorded.
Population measurement of ARK-1 and Ti To monitor the populations of ARK-1 and Ti, treatments (i), (ii), (iii), and (iv) were performed by using the antibiotic-resistant mutants ARK-1sc and VAT03-9n (Fig. S1, Table 1). In the ARK-1 migration assay in grapevine seedlings, ARK-1sc was inoculated into the middle position. To determine the bacterial population, stem parts (ca. 0.2 g fresh weight per plant, 1 sample per plant) were collected from ve plants (i.e., n = 5). Then each sample was scrubbed by hand under running tap water for 10 s, and the water drops were wiped off with paper towels. The samples were crushed in 1 mL of sterile distilled water using an autoclaved mortar and pestle. Ten-fold serial dilutions (100 μL) of each sample were prepared and spread on PSA media containing antibiotics. The plates were incubated at 25°C for 6 d, and the numbers of colony-forming units (CFU) were counted.

Gene expression analysis
For the gene induction assay shown in Fig. 3, ARK-1, Ti, or water (ca. 0.2 g) was inoculated into the middle position of seedling stems and shoot parts 5 mm away from the inoculation site and collected from three plants at 12,24,48, and 72 hpi. For the priming assay shown in Fig. 4, each bacterium was inoculated as treatment (iii) or (iv) (Fig. S1, Table 1). Shoot samples were collected as mentioned above at 24, 48, and 72 hpi. Total RNA was extracted from the frozen samples using the NucleoSpin RNA (Macherey-Nagel, Düren, Germany). To remove the genomic DNA in the extracted RNA and synthesize cDNA from 1.0 μg of total RNA, we used ReverTra Ace qPCR RT Master Mix with gDNA Remover (Toyobo, Osaka, Japan). Quantitative real-time polymerase chain reaction (qPCR) was carried out using Brilliant III Ultra-Fast SYBR Green QPCR Master Mix With Low ROX (Agilent, Santa Clara, CA, USA) and an AriaMx Real-Time PCR System (Agilent) with speci c primers for pathogenesis-related genes (PR-1 and PR-4), plant defensin 1.2 (PDF1.2), lipooxygenase 9 (LOX-9), and ethylene-responsive transcription factor ERF003 (ERF) [39][40][41][42] (Table S2). PR genes were used as a marker of SA signaling. and PDF1.2 and LOX-9 were used as markers of jasmonic acid (JA) signaling. ERF was used as a marker of ethylene (ET) signaling. The PCR conditions were 95°C for 10 min, followed by 50 cycles of 95°C for 15 s and 60°C for 1 min. Each sample was examined with three technical replicates, and dissociation curves were analyzed to verify the speci city of each ampli cation reaction. Cycle threshold values were calculated using AriaMx software version 1.5 (Agilent). The relative expression of each gene was obtained according to the Pfa equation 43 using actin as a reference gene 44,45 . Relative expression rates were calculated in comparison with values of the expression level of each gene at 12 or 24 hpi as 1.0 for Fig. 3 and Fig. 4, respectively. The experiments were performed 3 times for each assay.

Data analysis
Tukey's honestly signi cant difference (HSD, a= 0.05) test (after analysis of variance, ANOVA) was used to compare the CFU/g of plant tissue, relative gene expression, and gall size in the various treatments. Ryan's multiple-comparison (a= 0.05) test was used to compare the frequency of tumor formation among treatments. All statistical analyses were performed using version 3.6.1 of the R software (http://www.rproject.org/).

ARK-1 suppressed Ti-induced gall formation in positions distant from the inoculated site
To evaluate the biocontrol performance of ARK-1 at a position distant from the inoculation site, we inoculated grapevine stem at 3 inoculation sites (upper, middle, and lower) at 3 cm intervals (Fig. S1). We inoculated cell suspensions of Ti and ARK-1 into grapevine seedling stems with different combinations of timing, and then measured gall incidence (Fig. 1A) and gall size (Fig. 1B) at each point after 5 months. When Ti was inoculated into the middle position and water was inoculated into both upper and lower positions at the same time (treatment (i)) ( Fig. S1), galls were formed at all inoculation sites with an incidence of 100% (Fig. 1A). Each gall at the upper and lower positions was 2.58 and 2.89 mm, respectively, and both sizes were signi cantly smaller than that at the middle position (3.83 mm) (Figs. 1B and 2A). This result indicated that Ti moved 3 cm and produced galls at the position if it was wounded. Then, we inoculated Ti into the middle position and ARK-1 into both upper and lower positions at the same time (treatment (ii)) (Fig. S1). In this case, galls were formed only at the middle positions with 100% incidence (Fig. 1A). Their sizes were similar to those in the middle position of treatment (i) (Fig. 1B).
In this case, almost no galls were observed at either upper or lower positions (average gall incidence was 3.33%) (Figs. 1A and 2B). This meant that ARK-1 suppressed the virulence of Ti at the upper and lower positions but it had no effect on the distant positions when ARK-1 and Ti were inoculated together. Next, we inoculated water into both upper and lower positions, and Ti was inoculated at the middle position 5 days later (treatment (iii)) (Fig. S1). The result was similar to that of the treatment (i). Finally, ARK-1 was inoculated into both upper and lower positions, and Ti was inoculated into the middle position after 5 days (treatment (iv)) (Fig. S1). The gall formations were suppressed at the upper and lower positions (gall incidences were 3.33% and 0.00%, respectively) as observed in treatment (ii) (Fig. 1A). Interestingly, the gall incidence at the middle position was 60.00%, which was 40.00% lower than that in treatment (iii) and its gall sizes were signi cantly smaller (Figs. 1A and 1B). These results implied that ARK-1 could move at least 3 cm in 5 days and suppress the virulence of Ti. Note that no galls were found when water alone was inoculated as the negative control (data not shown).

ARK-1 migrated in grapevine seedling stem
To further con rm the possibility that ARK-1 moves 3 cm in 5 days in grapevine stems, the population of ARK-1 was measured in the region distant from the inoculation point. For this purpose, the spontaneously emerged antibiotic-resistant ARK-1 mutant (ARK-1sc) was used. ARK-1sc is resistant to both streptomycin and CuSO 4 . We inoculated a cell suspension of ARK-1sc into the middle position in grapevine seedling stems, and the inoculation and the upper and lower sites 3 cm away from the inoculation were sampled.
The bacterial concentrations in the extracts of these plant tissues were measured by counting colonies grown on a PSA medium containing the antibiotics. At the inoculation point, 5,623,413 CFU/g was detected ( Table 2). On the other hand, 426,579 and 79,432 CFU/g were detected in the upper and lower inoculation positions, respectively ( Table 2). They corresponded to 7.5% and 1.4% of the population in the inoculated point. This result showed that ARK-1 can migrate at least 3 cm to both upward and downward directions in 5 days through grapevine stems after inoculation.
Defense-related genes were induced 2-3 days after inoculation of ARK-1 and Ti Anand et al. 46 reported that SA and SAR play major roles in the resistance of Nicotiana benthamiana to R. radiobacter (Ti) (= A. tumefaciens (Ti)). Hao et al. 47 reported that R. radiobacter (Ti) induced the PR-1 gene in peach. Based on these ndings, we speculated that increased defense such as SAR or ISR in host plants is part of the biocontrol activity of ARK-1. To verify this possibility, expressions of defense-related marker genes in grapevine were monitored after the inoculation of ARK-1 or Ti. In this study, we used PR-1 and PR-4 for SA, PDF1.2 and LOX-9 for JA, and ERF for ET as marker genes for defense-related phytohormones [40][41][42] . Each bacterial strain was inoculated into stems of grapevine seedlings and plant tissues 5 mm from the inoculation points and sampled at 12, 24, 48, and 72 hpi. As a result, an increase (6-100 fold) of the expressions of PR-1, PR-4, LOX-9, and ERF was detected at 72 hpi upon the inoculation of both bacterial strains compared with the water control (Fig. 3). The expressions of PDF1.2 seemed to be slightly increased from 24 hpi, but the increases were small and unclear (Fig. 3). These results indicated that R. vitis could upregulate some kinds of defense responses possibly related to SA, JA, and ET in the surrounding area of the inoculation site in grapevine at 72 hpi regardless of its virulence.

Pre-inoculation of ARK-1 enhanced LOX-9 gene expression upon Ti inoculation
We examined whether the pre-inoculation of ARK-1 can make the plants more sensitive to subsequent pathogen infection during defense induction. We inoculated ARK-1 or water into both upper and lower positions on stems of grapevine seedlings as treatment (iv), and Ti was inoculated to the middle position after 5 days. Plant tissues 5 mm away from the Ti-inoculation point were sampled at 24, 48, and 72 hpi for further analysis of gene expression. PR-1, PR-4, PDF1.2, and ERF were upregulated at 72 hpi in response to the inoculation of Ti when water was pre-inoculated to the upper and lower positions. This was basically consistent with the results obtained without the pre-inoculation, as demonstrated in Fig. 3, although PDF1.2 expression was relatively higher (Fig. 4). In contrast, the expression levels of PR-4 and ERF at 72 hpi and PDF1.2 at 36 and 72 hpi after the Ti inoculation in the ARK-1-pretreated condition were decreased compared with those of the water-pretreated experiment. These results showed that ARK-1 seemed not to induce typical SAR or ISR, unlike the previously characterized bacterial biocontrol agents such as Pseudomonas uorescens. However, LOX-9 gene was induced by Ti at 24 and 48 hpi only when ARK-1 had been pre-inoculated into the distant position 5 days before. The expression of a particular range of defense genes may be primed by ARK-1.

Discussion
Our inoculation system with separate inoculation sites in the grapevine shoot revealed the migration capacities of ARK-1 and Ti. Ti could move at least 3 cm within 5 days and produced galls at that position if the site had been injured. Because the recognition of phenolic molecules such as acetosyringone is required for triggering of the virulence program in Rhizobium/Agrobacterium, such compounds should still remain at the wound site even after 5 days. This is basically consistent with the previous report showing that R. vitis (Ti) moved to 30 cm away from the entry point within 24 hpi 31 . On the other hand, Ti did not produce galls when it translocated to the site where ARK-1 was pre-inoculated. As we have already reported 25 , this result supports the usefulness of the pretreatment method of grapevine roots with the ARK-1 cell suspension before transplantation to control crown gall disease. In this study, the migration of ARK-1 along with the grapevine seedling stem was demonstrated in a manner similar to that of Ti. The ARK-1 cell density at the upper position 3 cm away from the inoculation point was higher than that of the lower position when ARK-1 had been inoculated into the middle position 5 days before. It may be easier to move upward than downward. ARK-1 translocated at least 3 cm within 5 days as well as Ti, and the gall incidence dropped by 60% at the site. This means that ARK-1 could exert its protective effect at the distant position, but it was still insu cient for full suppression. This would be due to the cell density. The ARK-1 populations at both upper and lower positions 3 cm away from the inoculation site at 5 dpi were 7.5 and 1.4% of that at the inoculation point, respectively. In other words, even small numbers of ARK-1 could work to a certain extent. We previously demonstrated that ARK-1 was effective in preventing gall formation on grapevine shoots when it was co-inoculated with Ti strains at a 1:1 cell ratio 16,27 . Although the effective concentration of ARK-1 is now being investigated, in the case of R. vitis VAR03-1 gall formation was suppressed when it was inoculated with the pathogen at a 1:1 ratio, but its control activity was decreased at 1:3 or 1:9 ratios 15 . Given the results obtained so far, in terms of practical usage of ARK-1 as a biocontrol agent for the management of crown gall disease in grapevine, we should allow a su cient period of time after pretreatment of grapevine shoots with ARK-1 in a non-contaminated place before transplanting them to the eld to wait for the bacterial density to be high enough. In addition to this pre-inoculation method, our results also showed the potential of ARK-1 treatment of growing grapevine trees in the eld. Although there is currently no practical way to save grapevine trees from crown gall disease in a pathogen-contaminated eld, inoculated ARK-1 may spread throughout whole plants gradually and protect them. Further investigation is needed to clarify if ARK-1 can translocate over long distances and suppress Ti-induced galls at places distant from the entry point in mature grapevine trees.
In this study, we tried to con rm the possibility of the involvement of increased defense in the biocontrol activity of ARK-1. The selected defense marker genes, PR-1, PR-4, LOX-9, PDF1.2, and ERF, for SA, JA, and ET were increased over 3 days after the inoculation of ARK-1 or Ti near the inoculation point (Fig. 3). This result indicates that grapevine induced defense responses to these bacteria. However, such defense responses were not detected at the ARK-1 inoculation point on the sixth day (Fig. 4). Therefore, the response to these bacteria would be diminished after 6 days. These results indicate that the direct induction of defense responses in host plants would not be the major factor in the ARK-1 biocontrol activity. The induction patterns of defense genes, PR-1, PR-4, EFF, and PDF1.2, upon Ti inoculation at the ARK-1 pre-inoculation points were similar to those to ARK-1 or Ti inoculation without pre-inoculation (Figs. 3 and 4). This also supports the idea that the defense responses have already decreased by the initial inoculation. The expressions of these genes were not accelerated and enhanced, suggesting that at least typical SAR and ISR may not be mounted by ARK-1. However, an unexpected response was detected in LOX-9. The LOX-9 gene was induced at 24 and 48 h after Ti inoculation only in the ARK-1 pre-treated plants. This result suggested that ARK-1 might facilitate the expression of a particular gene(s). LOX is known to be involved in the production of oxidized fatty acids in plants that can be the precursor of antibiotic compounds or signal molecules such as oxylipins 41,48,49 . The activation of systemic resistance by nonpathogenic rhizobacteria, Bacillus spp. and Pseudomonas putida, has been associated with the induction of LOX activity in bean and tomato 50 . Although the biological role of LOX-9 gene used in this study is unknown, it may somehow contribute to the ARK-1 biocontrol activity. Further transcriptome analysis could help clarify the role of this unique priming activity in its suppressive activity for crown gall disease. Rhizobium vitis strain VAR03-9 was used as Ti. In treatments (i) and (ii), all positions were inoculated at the same time. In treatments (iii) and (iv), Ti was inoculated 5 days post-inoculation (dpi) of water or ARK-1 at both upper and lower positions. For population assays, the antibiotic-resistant mutants ARK-1sc and VAT03-9n were used.      Induction of defense-related genes by ARK-1 and Ti during 3 days post-inoculation in grapevine seedlings. ARK-1, Ti, or sterile distilled water was inoculated into the middle position, and tissues 5 mm away from the inoculation sites were collected at the indicated time points. The relative expression rates of defense-related genes PR-1 (A), PR-4 (B), LOX-9 (C), PDF1.2 (D), and ERF (E) were measured using reverse transcriptase quantitative polymerase chain reaction (RT-qPCR) with speci c primers. Data are means ±SEM of relative expression rates to each value with water at 12 hours post-inoculation (hpi), which had a value of 1.0 (n = 3). Different letters represent signi cant differences according to Tukey's HSD (P ≤ 0.05). The experiments were repeated 3 times with similar results.

Figure 3
Induction of defense-related genes by ARK-1 and Ti during 3 days post-inoculation in grapevine seedlings. ARK-1, Ti, or sterile distilled water was inoculated into the middle position, and tissues 5 mm away from the inoculation sites were collected at the indicated time points. The relative expression rates of defense-related genes PR-1 (A), PR-4 (B), LOX-9 (C), PDF1.2 (D), and ERF (E) were measured using reverse transcriptase quantitative polymerase chain reaction (RT-qPCR) with speci c primers. Data are means ±SEM of relative expression rates to each value with water at 12 hours post-inoculation (hpi), which had a value of 1.0 (n = 3). Different letters represent signi cant differences according to Tukey's HSD (P ≤ 0.05). The experiments were repeated 3 times with similar results.