Biocontrol Potential of Purified Elicitor Protein PeBL1 Extracted from Brevibacillus laterosporus Strain A60 and Its Capacity in the Induction of Defense Process against Cucumber Aphid (Myzus persicae) in Cucumber (Cucumis sativus)

The Cucumber aphid (Myzus persicae), a destructive cucumber aphid usually managed by chemical pesticides, is responsible for enormous annual agricultural losses. A protein elicitor, PeBL1, was investigated in the present work for its ability to induce a defense response against M. persicae in cucumber. The rates of population growth (Intrinsic rate of increase) of M. persicae (second and third generations) decreased with PeBL1-treated cucumber seedlings as compared to positive (water) and negative 70.58 μg mL−1 controls (50 mM Tris-HCl, pH 8.0). In an assay on host selection, M. persicae had a preference for colonizing control plants as compared to the PeBL1-treated cucumber seedlings. The nymphal development time of the aphid was extended with the PeBL1-treated cucumber seedlings. Likewise, fecundity was reduced, with less offspring produced in the PeBL1-treated cucumber seedlings as compared to the positive (water) and negative 70.58 μg mL−1 controls (50 mM Tris-HCl, pH 8.0). The cucumber leaves treated with PeBL1 had a hazardous surface environment for M. persicae, caused by trichomes and wax formation. Jasmonic acid (JA), salicylic acid (SA), and ethylene (ET) levels were significantly higher, exhibiting significant accumulation in the PeBL1-treated cucumber seedlings. The following results showed that PeBL1 considerably altered the height of the cucumber plant and the surface structure of the leaves to minimize M. persicae reproduction, and it prevented colonization. Defensive processes also included the activation of pathways (JA, SA, and ET). This study provides evidence of biocontrol for the use of PeBL1 in cucumber defense against M. persicae.


Introduction
A multifaceted relationship has been established between herbivores and plants during development. Plants damaged by herbivores show the accumulation of toxic or volatile organic compounds with the modification of their physical structures. The structures and compounds affect the growth, colonization, feeding, survival, and oviposition of herbivores, and they attract natural enemies and encourage them to induce defense [1]. In order to deal effectively with this damage, two mainly constitutive defense mechanisms have been developed by plants [2]. Plants are prevented from

Aphid and Plant Preparation
Myzus persicae (Sulzer), commonly known as the green peach aphid, was collected from the cucumber field at the Chinese Academy of Agricultural Sciences in Beijing, China, and transferred to cucumber seedlings (Cucumis sativus). The aphid was reared in a chamber with 16 were sterilized with 75% ethanol over 15-20 s and washed with distilled water, and then they were pre-soaked in distilled water 2-3 days before use.

Evaluation of PeBL1
PeBL1 was produced with the recombinant vector pET30-TEV/LIC in Escherichia coli BL21-DE3 (Novagen, Darmstadt, Germany). The pellets were removed, and the supernatant cells were resuspended and sonified by the ultrasonic disruptor. The supernatant was collected and filtered with filter paper (size 0.22 µm) after the solution was centrifuged at 12,000 rpm for 15 min. The Äkta Explorer Protein Purification System (Amersham Biosciences, Temecula, CA, USA), as described by Wang et al. [21], with a His-Trap HP column (GE Healthcare, Waukesha, WI, USA), used various loading buffers (A, B, C, and D) for the further purification of the elicitor protein PeBL1. Buffer A (50 Mm Tris-HCl, 8.0 pH), washed off other elicitors from the column quickly, and buffer B was used to stabilize the column 200 Mm NaCl). For the solution elution elicitor protein, Buffer C (50 Mm Tris-HCl, 200 Mm NaCl, and 20 Mm imidazole, pH 8.0), and elusion Buffer D 200 Mm NaCl, and 500 Mm imidazole, pH 8.0). Then the PeBL1 elicitor protein was desalted in a HiTrap desalting column (GE Healthcare, Waukesha, WI, USA), as described by Wang et al. [21]. The molecular mass of the purified elicitor protein was measured by a 12% SDS-PAGE resolving gel, and a GenStar M223 protein marker (~5-245 kDa) was used for the estimation of the molecular mass of the purified PeBL1 elicitor.

The Population of M. persicae
Cucumber seeds and young seedlings were soaked for 24 h in four concentrations of the PeBL1 solution, i.e., 70. 58, 42.34, 21.17, and 17.64 µg mL −1 . Three seeds in a single pot were cultivated in organic soil (Flora Guard substrate). Three-week-old seedlings of cucumber with the different concentrations of the PeBL1 solution were sprayed after 7 days and then inoculated with 10-12 adults of M. persicae per plant after 24 h. For M. persicae, after inoculation, the number of settled aphids' population, was recorded after every 5 days as described by Li et al. [24]. Water and 70.58 µg mL −1 of a buffer (50 mM Tris-HCl, pH 8.0) were tested for positive and negative controls. A CRD randomized statistical design was used. Transparent air-permeable cages were used to separate seedlings from each plant. The experiment was conducted twice with four replications.

The Intrinsic Rate of Increase of M. persicae
Cucumber seeds were soaked in 70.58 µg mL −1 of a purified protein solution for 24 h and then transferred for sprouting 2-3 days in distilled water in petri plates. A CRD randomized statistical design was used. Seedlings were sprayed after 24 h with 70.58 µg mL −1 of the PeBL1 purified protein solution. Inoculation with a freshly born M. persicae nymph was then carried out for every seedling. A glass tube cotton-gauze was used to separate all seedlings. Twice a day, the new-born aphid was observed to record the total time and number of offspring produced, which were removed every day. The same test was conducted on seeds and seedlings after 5 days. The experiment was repeated twice individually, with 30 replicates per treatment. The increase in each aphid's intrinsic rate was measured by: Md is the number of nymph's new-born in the development time equal to T d , which is the time between an aphid's birth and its first reproduction

Feeding Preference of M. persicae Choice Test
Cucumber seeds and seedlings, as described in Section 2.2, were treated. The cucumber PeBL1-treated and control seedlings were put in a transparent breathable cage (60 × 60 × 60) cm with cross-touch leaves and a white cardboard bridge (12 × 4) cm connecting the base section of stems. A CRD randomized statistical design was used. Thirty wingless M. persicae adults in the center of the bridge were released. The experiment was repeated 15 times, and after 24 h, the aphids were counted on each seedling.

Detection of Aphid Feeding Activities by Electrical Penetration Graph (EPG)
As previously described, the cucumber seeds were soaked and germinated for 3-4 days in distilled water. Similarly, sized seedlings were then individually planted to organic soil until day 7. Twenty-four hours after the spraying of the seedlings, an electrical penetration graph (EPG; GIGA-8d) was used on wingless, 12-15-day-old, healthy adult M. persicae. Before the test, all aphids were starved for 1 h. The experiments were conducted daily for 4 h at the same time. An A B stylet was used for the determination and manual study of the aphid feeding waves. A wave identifier was previously described [25].

Aphid Bioassay
A bioassay of the PeBL1 elicitor was carried out with different concentrations of the protein purified solution, i.e., 70. 58, 42.34, 21.17, and 17.64 µg mL −1 , a positive control (water alone), and a negative control (70.58 µg mL −1 buffer) against M. persicae on the plants of cucumber. A Bradford assay was used to determine different protein concentrations. At the three-leaf stage of the cucumber plant, approximately 2-3 mL of PeBL1 was applied with a separate spray bottle until the solution drained off from plants. For positive and negative controls, waters and buffers (50 mM Tris-HCl, pH 8.0) were used. The plants were allowed to dry overnight, and 3-5 numbers of freshly molted 0-6 h aphids were allowed to feed on these plants. The time of nymph development was observed by consecutive observations at intervals of 3 h until the bioassays were completed for each instar as the total number of offspring produced by all aphid instars, while the number of days in which aphids lived was considered the longevity. Data were compared statistically by a factorial ANOVA and least significant difference (LSD) at α = 0.05. Bioassays were repeated independently at three non-identical temperature regimes (20,24,27 • C) by using 10 replicates per treatment.

Effect of PeBL1 on the Growth and Structure of Cucumber
Seven-day-old cucumber seedlings were treated in the same manner as above. One day after the seedlings were sprayed, the seeds were soaked for eight days. The central part for the first leaves was collected and tested, while 3.5% glutaraldehyde diluted into a 0.1 M phosphate buffer (pH 7.2) was used for sampling up to 48 h. For approximately 15 min, all samples were cleanly washed in a 0.1 M phosphate buffer (pH 7.2) and then submerged in 1 percent osmic acid for about 2 h five different times. A gradient of ethanol of 100, 95, 90, 80, 70, 60, 50, and 30% was used for 15 min. A Leica EM critical point dryer (CPD030; Leica Biosystems, Wetzlar, Germany) was used to dry all samples at critical points. A Hitachi H-7650 transmission electron microscope was used to monitor all samples, Total plant height (cm), total chlorophyll amount (SPAD), total fresh and dry weight, and the number of plant leaves, with 10 replicates per treatment, were measured in order to quantify the effect of PeBL1-treated settlements. A CRD randomized statistical design was used, and data were compared statistically by an ANOVA and LSD at α = 0.05.

HPLC/MS Detection of the Plant Hormone
As before, seeds and seven-day-old seedlings were treated. As mentioned above, approximately 0.5 g of the aerial part of the seedlings was collected to extract SA, JA, and ET [26]. A high-performing liquid chromatography spectrometer was used to inject some 20 µL of extraction (HPLC/MS; Shimazu Research Instruments, ODS-C18, 3 µm, 2.1 per 150 mm Kyoto, Japan). HPLC was performed at a flow rate of 0.2 mL min −1 with a mobile phase of 60% methanol, 40 • C column temperature, and 4 • C sample temperature. In the negative ion mode (SA m/z: 137.00; JA: 209.05) MS was set at the selected ion monitoring system (SIM) with a solvent temperature of 250 • C, a heat block temperature of 200 • C, Biology 2020, 9, 179 5 of 22 a drying gas flow rate of 10 L min −1 , a nebulizing gas flow of 1.5 L min −1 , a detector voltage of 1.30 kV, and an interface voltage of −3.5 kV.

Expression of the Gene by Q-RT-PCR
TransGen Biotech (Beijing, China) kits were used for extracting RNA, synthesizing cDNA, and conducting a quantitative polymerase chain reaction in real-time (RT-qPCR) (ABI 7500 Real-Time PCR System). The excellence of RNA was calculated with an NP80 nano-photometer. The tested JA, SA, and ET genes were ChIT1 (class III chitinases PR-3); β-1,3-Glucanase (beta-glucanase); PAL1 (phenylalanine ammonia-lyase); LOX1 (lipoxygenase multifunctional proteins), PR1 (pathogenesis-related to protein 1), cupi4 (cucumber pathogenesis-induced 4), and PR2 (pathogenesis-related to protein 2); the ribosomal gene 18S was considered as the internal reference gene [27]. The primers of all pathways are listed in Table A1 of Appendix A. The application of the 2 −∆∆CT was used to check the relative fold expression of the genes [28].

Analysis of Data
Data from two treatments were compared statistically using an independent Leven's test, and a two-tailed t-test and data obtained from three or more treatments were compared statistically by the LSD and an ANOVA. Statistix software version 8.1 (Analytical Software, Tallahassee, FL, USA) was used for statistical data analysis. Data on the fecundity of aphids were square-root transformed prior to analysis. In order to take out differences, a one-way factorial analysis of variance was performed among treatment factors such as the concentrations of PeBL1 elicitor and different temperature regimes, followed by the least significant difference test, at a probability of 95%. The expressions of genes (RT-qPCR) were obtained by the comparative CT (2 −∆∆CT ) method. The Student's t-test (p = 0.05) was used to compare fold changes in the plant samples treated with the elicitor and the buffer.

Expression, Purification, and Evaluation of PeBL1 Elicitor Protein
The PET30-TEV/LIC recombinant vector was transformed into E. coli BL21 (DE3) cells. The expressed His6-PeBL1 was soluble in E. coli after successful transformation. PeBL1 was purified with the column of the His-Trap HP (GE Healthcare, Waukesha, WI) ( Figure 1A) and was desalted, as previously described by Wang et al. [21], in the HiTrap column. A single band showed the characteristics of pure recombinant protein at 12 kDa on Tricine SDS-PAGE ( Figure 1B).

Myzus persicae Performance Indoors
PeBL1 induced resistance to cucumber aphid M. persicae in two separate ways. First, a settled aphid population decrease was observed in the PeBL1-treated cucumber seedlings (Table 1), and the percentage decreases in population count in PeBL1 treatment relative to the buffer and control treatments are indicated in Tables A2-A4 of Appendix B. M. persicae, in the host selection assay, preferred to feed on the control cucumber seedlings. A day after the inoculation of the aphid and two days after spraying of the seedlings, the amount of M. persicae colonizing PeBL1-treated plants was significantly lower than the control and "Elsewhere"-the latter of which is aphid colonization in places other than buffer-and PeBL1-treated areas (Table A5 of Appendix C). Based on their feeding behavior, some aphids showed colonization in areas opposite to that treated with buffer and PeBL1, (Figure 2A,B). Second, in the case of PeBL1 treatment, the developmental time of the cucumber aphid was extended more compared to the control, whereas the everyday reproductive abilities of M. persicae that were fed on seedlings treated with PeBL1 were reduced (second and third nymphal instars). Second and third generations experienced lower growth rates (Table 2). Biology 2020, 9, x FOR PEER REVIEW 6 of 24

Myzus persicae Performance Indoors
PeBL1 induced resistance to cucumber aphid M. persicae in two separate ways. First, a settled aphid population decrease was observed in the PeBL1-treated cucumber seedlings (Table 1), and the percentage decreases in population count in PeBL1 treatment relative to the buffer and control treatments are indicated in Tables A2-A4 of Appendix B. M. persicae, in the host selection assay, preferred to feed on the control cucumber seedlings. A day after the inoculation of the aphid and two days after spraying of the seedlings, the amount of M. persicae colonizing PeBL1-treated plants was significantly lower than the control and "Elsewhere"-the latter of which is aphid colonization in places other than buffer-and PeBL1-treated areas (Table A5 of Appendix C). Based on their feeding behavior, some aphids showed colonization in areas opposite to that treated with buffer and PeBL1, (Figure 2 A, B). Second, in the case of PeBL1 treatment, the developmental time of the cucumber aphid was extended more compared to the control, whereas the everyday reproductive abilities of M. persicae that were fed on seedlings treated with PeBL1 were reduced (second and third nymphal instars). Second and third generations experienced lower growth rates ( Table 2).    Note: Data are shown as mean ± SD. Data were compared statistically by an ANOVA and LSD in Statistix software, version 8.1. Significant differences can be seen in letters in rows at all treated samples after the inoculation of the aphid on the same day (p = 0.05).

M. persicae Feeding Behavior by EPG
An EPG provided a general illustration of the cucumber resistance factors. The feeding behavior of M. persicae in seedlings treated with PeBL1 was significantly altered. EPG data (Table 3) showed that the probing period, the length of C (pathway operation in all tissues), and the sum of M. persicae Pd (potential decrease in cell punctures) were significantly reduced, whereas the period of non-probe time before the first E (phloem-feeding activity) and the total duration of F (penetration problems) in the PeBL1-treated cucumber seedlings increased considerably. No electrical contact between the aphid stylet and the plant was indicated during the non-probing time [29]. In the PeBL1 treatment, the non-probing time before the first E was dramatically increased, suggesting a repellent or deterrent surface factor in the PeBL1-treated cucumber seedlings. C waves represent style motion in intercellular Biology 2020, 9, 179 8 of 22 space and may constitute a plant mechanical barrier [30]. The shorter C waves (<3 min) that were detected, the greater the mechanical difficulty in seedlings treated with PeBL1. Additionally, a lower Pd number (cell puncture) was associated with the plant's aphid resistance, which could have been due to mechanical difficulty (in this study, in the PeBL1-treated cucumber seedlings). The wave E1 (saliva injection during phloem-feeding activities) indicated saliva injection by aphids into sieve elements. In contrast, the E2 wave (sap-sucking during phloem-feeding activities) showed phloem sap injection with concurrent salivation, which could have reflected a mesophyll or vascular resistance factor [31]. In the sieve element [24,31] the extended E1 indicated more plugging or defense compounds. There was, however, no substantial difference between the control and PeBL1 treatments in the E2 period, indicating no or low variability in phloem compounds to confer resistance to M. persicae. However, the period of the F wave in the PeBL1-treated cucumber seedlings was higher, indicating that PeBL1 induced an enhanced mechanical defense. The EPG results suggested that the resistance induced by PeBL1 was mainly due to the modification of the physical defense. Note: Data are shown as mean ± SD. C stands for pathway activities, Pd stands for potential drop, E stands for phloem-feeding activities, F stands for penetration problem, G stands for xylem feeding activities, E1 stands for saliva injection, and E2 stands for sap-sucking. Data were compared statistically by an independent t-test with two tails and Levene's test in Statistix, version 8.1. Asterisks indicate significant differences between PeBL1 treatment and control with the same parameters of * (p = 0.05).

Impact of PeBL1 Elicitor on Aphid's Nymphal Development Time
Factorial analysis showed an impact on the overall developmental time of M. persicae on various PeBL1 concentrations in three different temperature regimes and their interaction. A differential trend was identified on the developmental time of nymphs for the elicitor effect at a different temperature, as shown in Tables A6-A10 of Appendix D. With increasing concentrations of PeBL1, ( Figure 3A) the development time of each nymphal instar was extended. For the fourth nymphal instar at a high concentration (70.58 µg mL −1 ), the maximum development time was 3.7 d at the low temperature of 20 • C. At the low concertation (17.64 µg mL −1 ) for the first instar at the high temperature of 27 • C, the minimum nymph growth time was recorded. The time of nymph development ( Figure 3B) differed in the buffer control and water-treated control. In general, the nymphal development time of all instars at the low temperature was higher than at medium or high temperatures. At each concentration and temperature of the elicitor, the maximum elongation of time was observed at fourth instar. However, for the first, second, third, and fourth instar aphid concentration of the elicitor, PeBL1 showed significance. Likewise, the effect of temperature regimes also had a significant impact on the developmental time of nymph of the first, second, third, and fourth instar aphids. Afterwards, nymphal aphid development time showed little difference across their shared interface. After all, the nymphal development time did not show any fluctuation with their mutual interaction. development ( Figure 3B) differed in the buffer control and water-treated control. In general, the nymphal development time of all instars at the low temperature was higher than at medium or high temperatures. At each concentration and temperature of the elicitor, the maximum elongation of time was observed at fourth instar. However, for the first, second, third, and fourth instar aphid concentration of the elicitor, PeBL1 showed significance. Likewise, the effect of temperature regimes also had a significant impact on the developmental time of nymph of the first, second, third, and fourth instar aphids. Afterwards, nymphal aphid development time showed little difference across their shared interface. After all, the nymphal development time did not show any fluctuation with their mutual interaction.

Effect of PeBL1 Elicitor on the Aphid's Fecundity
The figures show that the concentrations of PeBL1 (F 5.162 = 83.82; p < 0.0001) and temperature regimes (F 2.162 = 8.97; p < 0.0002) were significantly affected by aphid fecundity, as shown in Appendix E of Table A11. (Figure 4A,B) shows that M. persicae produced less offspring than those that feed on (water) positive and (buffer) negatively treated cucumber plants in contrast to the PeBL1-treated seedlings ( Figure 5). However, a minimum fecundity at a maximum temperature was observed at 27 • C, and a maximum fecundity at a minimum temperature of 20 • C was recorded.

Effect of PeBL1 on the Growth and Structure of Cucumber
The plant height and surface structure of the cucumber leaves were greatly modified by PeBL1 ( Figure 6). A similar trend was also found in the SPAD, the total number of leaves, and plant fresh and dry weight (Tables A12-A16 of Appendix F). In PeBL1-treated seedlings, plant height was greater than that of the control. The surface of cucumber leaves was significantly modified by PeBL1 elicitor protein, seedlings treated with PeBL1 exhibited more trichomes as compared to control in PeBL1 treated 60.84 ± 0.52 mm −2 , while in control treatment it was 34.30 ± 0.10 mm −2 . A more sophisticated wax structure was formed that gave rise to a significantly better surface environment, one that trait is considered to be unfavorable to aphid settlement [32].

Effect of PeBL1 Elicitor on the Aphid's Fecundity
The figures show that the concentrations of PeBL1 (F5.162 = 83.82; p < 0.0001) and temperature regimes (F2.162 = 8.97; p < 0.0002) were significantly affected by aphid fecundity, as shown in Appendix E of Table A11. (Figure 4 A, B) shows that M. persicae produced less offspring than those that feed on (water) positive and (buffer) negatively treated cucumber plants in contrast to the PeBL1-treated seedlings ( Figure 5). However, a minimum fecundity at a maximum temperature was observed at 27 °C, and a maximum fecundity at a minimum temperature of 20 °C was recorded.

Effect of PeBL1 on the Growth and Structure of Cucumber
The plant height and surface structure of the cucumber leaves were greatly modified by PeBL1 ( Figure 6). A similar trend was also found in the SPAD, the total number of leaves, and plant fresh and dry weight (Tables A12-A16 of Appendix F). In PeBL1-treated seedlings, plant height was greater than that of the control. The surface of cucumber leaves was significantly modified by PeBL1

SA, JA and ET Accumulations in PeBL1-Treated Cucumber Seedlings
To analyze the relation of JA, SA, and ET with the cuticular wax deposition and increase in the trichome density of PeBL1, the aphid infestation or both were analyzed. PeBL1 showed a very high

SA, JA and ET Accumulations in PeBL1-Treated Cucumber Seedlings
To analyze the relation of JA, SA, and ET with the cuticular wax deposition and increase in the trichome density of PeBL1, the aphid infestation or both were analyzed. PeBL1 showed a very high accumulation of JA, SA, and ET in seedlings (Figure 7). All three pathways of signaling were found to participate in aphid-induced cucumber resistance [33]. In addition, JA, SA, and ET accumulated in PeBL1-treated plants, suggesting that the protein elicitor at least partially induced the defense response in cucumber plants. Numbers, infestation rates, and aphid species are known to affect JA, SA, and ET inductions [34,35].
Biology 2020, 9, x FOR PEER REVIEW 13 of 24 accumulation of JA, SA, and ET in seedlings (Figure 7). All three pathways of signaling were found to participate in aphid-induced cucumber resistance [33]. In addition, JA, SA, and ET accumulated in PeBL1-treated plants, suggesting that the protein elicitor at least partially induced the defense response in cucumber plants. Numbers, infestation rates, and aphid species are known to affect JA, SA, and ET inductions [34,35].

Relative Fold Expressions of Defense-Related Genes
PeBL1 enhanced the defense mechanism in cucumber seedlings. ChIT1, β-1,3-Glucanase, PAL1, LOX1, PR1, cupi4, PR2, and Pod were selected as test genes for defense pathways. All the genes were up-regulated by treatment with PeBL1 and aphid infestation ( Figure 8); the transcripts of all genes were found to be statistically greater with the PeBL1 treatment than with the other two treatments. The idea was that PeBL1 treatment enhanced induced resistance to aphid infestation. The improved transcript of test genes of JA and SA also demonstrated their roles for the JA and SA pathways in aphid resistance in wheat, which was proven by Moron and Thompson. The highest expressed gene was ChIT1, followed by β-1, 3-Glucanase, PR1, LOX1, PAL1, cupi4, PR2, and Pod. The Log2 of all JA, SA, and ET test genes was computed with fold change expression values (Table 4) showed that aphid resistance was due to the transcription of the test genes. , and ethylene (ET) contents in cucumber seedlings (mean ± SD). Treatment with PeBL1 was collected one day after spraying. In both treatments, the aphids were inoculated one day after seedlings were sprayed, and the samples were collected one day after inoculation. Data were compared statistically by the LSD, ANOVA, and Leven's test using Statistix, version 8.1. Different lower-case letters show significant differences among various treatments performed in JA, SA, or ET (p = 0.05).

Relative Fold Expressions of Defense-Related Genes
PeBL1 enhanced the defense mechanism in cucumber seedlings. ChIT1, β-1,3-Glucanase, PAL1, LOX1, PR1, cupi4, PR2, and Pod were selected as test genes for defense pathways. All the genes were up-regulated by treatment with PeBL1 and aphid infestation ( Figure 8); the transcripts of all genes were found to be statistically greater with the PeBL1 treatment than with the other two treatments. The idea was that PeBL1 treatment enhanced induced resistance to aphid infestation. The improved transcript of test genes of JA and SA also demonstrated their roles for the JA and SA pathways in aphid resistance in wheat, which was proven by Moron and Thompson. The highest expressed gene was ChIT1, followed by β-1, 3-Glucanase, PR1, LOX1, PAL1, cupi4, PR2, and Pod. The Log 2 of all JA, SA, and ET test genes was computed with fold change expression values (Table 4) showed that aphid resistance was due to the transcription of the test genes.

Discussion
The use of elicitors is a new biological tool for the management of insect pests, as they play a dynamic role in the defense and signaling mechanisms of plants under the attack of sap-feeding insects [17,19,20], Numerous B. laterosporus strain have demonstrated various broad-spectrum anti-microbial activities, acting as anti-microbial peptides in microbes such as bacteria and fungi. They can enter into the cell and transfer to the cytoplasm and nucleus to interrupt protein synthesis by mixing up DNA and RNA [36,37]. A significant source of elicitors such as PAMPs or MAMPs [38] is pathogenic bacteria and fungi, whether necrotrophic or biotrophic. The potential activities of PeBL1 derived from B. laterosporus strain A60 were demonstrated in this study for M. persicae management. Certain studies have previously shown chemical elicitors significantly reduced the activity of herbivorous pests in cucumber crops by applying chemical elicitors, such as methyl-jasmonate, benzothiadiazole, and other plant defenses, including proteinase inhibitors [39]. Results from this study confirmed previous results that the use of methyl salicylate elicitor reduced the soybean aphid Aphis glycines by up to 40% [38,39]. Here, bioassays showed that population development on PeBL1-treated cucumber plants was significantly slower compared to the buffer and control. Previous studies have shown a negative influence of exogenous applications of elicitors, including MJ, JA, and BTH, on the population growth and fitness of different aphid species, an effect confirmed by the present findings [39]. Similarly, a biocontrol potential was discovered against various Diptera, Coleoptera, and Lepidoptera, as well as against nematodes and mollusks [23,40]. The current study showed the ability of PeBL1 to suppress herbivores by influencing population and growth parameters. Trichomes are the first lines of physical resistance to pathogenic microorganisms and herbivores. These hairy adjuncts of plant epidermal cells affect the herbivores' morphology and the density role of trichomes in Solanum spp., i.e., seven trichomes with two major defense-related effects, have been tested [40]. First, a plant surface represents a physical barrier because its thick matte hair provides energy, limits feeding capacity, and reduces access to the surface by insects. Excessively hairy plants, such as Solanum hirsutum, are avoided by M. persicae. Trichomes are also associated with the basic defensive mechanism of the tomato plant, as the surface area covered by the epidermal cell appendages of unicellular or multicellular hairs provide resistance to a variety of pests due to the "pubescence" of a plant. Leaf beetle (Coleoptera: Chrysomelidae) settlement with thick trichomes was reduced in soybeans compared with the trichome-removed plants, which attracted more beetles [41][42][43]. PeBL1 reduced disease severity, triggering a photosynthesis process that mirrored the characteristics of growth of plants [44], and it enhanced induced-resistance in the PeBL1-treated cucumber seedlings as well.
Compared to the controls, the PeBL1-treated seedlings and leaves had more trichomes. The PeBL1-treated cucumber seedlings and leaflets were reported to have inhibited the reproduction and settlement of aphids with an increased number of trichomes. The feeding activity of Leptinotarsa decemlineata was negatively affected by a high density of trichomes. Another key part of physical barrier lignin is the cell wall, which underpins plant resistance and is an indicator for the improvement of the cell wall [45]. Aphid tolerance in chrysanthemum was amended by an enhanced lignin content [46]. The physical defenses of plants include, in response to biotic and abiotic stress, trichomes and wax production. Their establishment can be induced by direct damage, e.g., as induced by leaf-cuts, methoxyfenozide, and manganese [47,48]. The use of exogenous phytohormones, MJ, or JA can also affect cuticular wax deposition and trichome density, as shown in Arabidopsis and tomatoes, respectively [49]. The SA application was due to wax deposition in Brassica napus [50]. Accumulations of SA and JA in PeBL1-treated cucumber plants can, therefore, be hypothesized as being related to increased trichome density and the deposition of cuticular wax. In addition, the treatment of the PeBL1 elicitor had adverse effects on aphid fecundity. PeBL1-treated plants produced significantly fewer aphids than the buffered and controlled seedlings. The results were consistent with previous studies showing that exogenous SA and MJ have caused lower mean lifetime fecundity in aphids [38]. Therefore, optimum temperatures (e.g., 24 • C) demonstrated a maximum aphid fecundity, with the minimum fecundity at higher temperatures (27 • C) due to a decreased metabolic rate [51]. Similarly, a variance analysis showed that in PeBL1-treated plants, the development time of nymphs was extended compared to the control; even at a lower temperature (20 • C), the maximum nymphal development time was observed, indicating that a one-degree temperature increase affected the life cycle of the insect [52]. Additional studies need to be conducted to understand the underlying mechanism of PeBL1 in cucumbers, in particular its effect on fecundity and nymphal development time.
Additionally, JA, SA, and ET increased marker gene transcriptions, signaling that they play an essential role in cucumber aphid resistance. After aphid infestation in Arabidopsis, the transcript genes CHIT1, β-1,3-glucanase, PR1, LOX1, PAL1, cupi4, PR2, and Pod were significantly increased. Actin is a structural component in the plant cell wall that is depolymerized via the regulation of cell and cross-linking [53,54]. Actin depolymerization is negatively related to aphid fecundity and population [55]. JA, SA, and ET molecules impart resistance to insect herbivorous diseases and pathogens, which enhances plant defense responses [12,[56][57][58]. All JA, SA, and ET test genes showed significant and robust regulation [12]. PAL1 coding for ammonia-lyase phenylalanine is involved in cell wall construction, as demonstrated in Arabidopsis [59]. JA and LOX1 up-regulation occur in cucumber plant Pseudomonas injection [59,60]. PR1 and PR2 are systemically acquired (SAR) pathogenesis-related proteins [13,61,62]. Cupi4 genes with antibacterial characteristics also lead to the induction of hypersensitive reactions in the infected tissues of plants [63,64]. The presence of CHIT1 (PR-3 family) genes indicates fungal cell wall damage in plants due to antifungal activity [13,65]. β-1, 3-Glucanase (beta-glucanase) codes show a plant-friendly defense mechanism against several microorganisms, as well as an increase in β-1,3-glucanase in P. melonis fungal cell walls, which leads to the inhibition of disease growth in infected plants [66,67]. Pod codes peroxidase, which indicates that the acclimation of the Pod will mediate aphid resistance in cucumbers [68]. Experimental findings from this research confirm that the activation of Pod by M. persicae induces genes associated with the defense pathway [69].

Conclusions
Herein, we present data on aphid resistance in cucumbers with the prolonged developmental time of the first to fourth nymphal instars, related to a lower fecundity of M. persicae. Increased PeBL1 concentrations were found to affect aphid colonization. The resistance factors were verified by the increased number of trichomes and wax amounts, which were mainly involved in mechanical defenses. Likewise, an EPG study confirmed that the resistance induced by PeBL1 was mainly due to the modification of the physical defense and increased number of trichomes, and wax composition affected aphid feeding behavior in PeBL1-treated. Moreover, our study focused on the effect of PeBL1 on the growth and structure of cucumber, and we found that increased plant height and modified surface structures of the cucumber leaves were greatly influenced by PeBL1. We also confirmed the role of PeBL1 in physical defense against M. persicae. The physical defense response induced by PeBL1, JA, SA, and ET contributed to a comprehensive plant physical response.
However, some issues need to be resolved in the future, e.g., "how JA, SA and ET work resistance induction," and "whether or not other plant hormones are involved." Nevertheless, the current study showed that PeBL1 isolated from B. laterosporus A60 strain could be applied to cucumber seed and seedlings to protect plants against M. persicae.