Silicon Dioxide Nanoparticles Induce Innate Immune Responses and Activate Antioxidant Machinery in Wheat Against Rhizoctonia solani

The phytopathogenic basidiomycetous fungus, Rhizoctonia solani, has a wide range of host plants including members of the family Poaceae, causing damping-off and root rot diseases. In this study, we biosynthesized spherical-shaped silicon dioxide nanoparticles (SiO2 NPs; sized between 9.92 and 19.8 nm) using saffron extract and introduced them as a potential alternative therapeutic solution to protect wheat seedlings against R. solani. SiO2 NPs showed strong dose-dependent fungistatic activity on R. solani, and significantly reduced mycelial radial growth (up to 100% growth reduction), mycelium fresh and dry weight, and pre-, post-emergence damping-off, and root rot severities. Moreover, the impact of SiO2 NPs on the growth of wheat seedlings and their potential mechanism (s) for disease suppression was deciphered. SiO2 NPs application also improved the germination, vegetative growth, and vigor indexes of infected wheat seedlings which indicates no phytotoxicity on treated wheat seedlings. Moreover, SiO2 NPs enhanced the content of the photosynthetic pigments (chlorophylls and carotenoids), induced the accumulation of defense-related compounds (particularly salicylic acid), and alleviated the oxidative stress via stimulation of both enzymatic (POD, SOD, APX, CAT, and PPO) and non-enzymatic (phenolics and flavonoids) antioxidant defense machinery. Collectively, our findings demonstrated the potential therapeutic role of SiO2 NPs against R. solani infection via the simultaneous activation of a multilayered defense system to suppress the pathogen, neutralize the destructive effect of ROS, lipid peroxidation, and methylglyoxal, and maintain their homeostasis within R. solani-infected plants.


Introduction
Wheat (Triticum aestivum L.) is an important cereal crop worldwide, which is considered stable food for about one-third of the world population. Wheat plays an important role in total cereal production and global food security [1]. It comes after rice and corn with respect to stable food for most of the world population. Rhizoctonia spp. is among various fungal pathogens that cause wheat diseases and affect wheat [2,3]. Two anamorph species of genus Rhizoctonia, which causes root disease on wheat and negatively affects its 2θ = 22.8 o and no additional peaks were observed by the XRD spectrum ( Figure 1B). The presence of SiO2 NPs was confirmed by exhibiting a peak at approximately 440 nm in UV-Vis spectra ( Figure 1C). The nanoparticles size ranged from 9.92 to 19.8 nm as obtained from TEM images ( Figure 1D). Obtained NPs were spherically shaped, which was detected by using TEM. Data from the energy dispersion spectrum (EDS) of Si Kα1 ( Figure  S1A), O Kα1 (Figure S1B), and SiO2 ( Figure 1E) showed that SiO2 NPs contained almost 2:1 oxygen and silicon, respectively (71% O and 29% Si; Figure 1F).

Responses of Wheat Cultivars to R. solani
The tested wheat cultivars showed variable responses to R. solani infection ( Figure 2). The tested isolate expressed symptoms of pre-, post-emergence damping-off and root rot on all wheat cultivars. The highest pre-emergence damping-off values were observed on wheat cvs. Giza-171 (30%), Giza-168 and Misr-1 (28%). However, a low percentage of pre-

Responses of Wheat Cultivars to R. solani
The tested wheat cultivars showed variable responses to R. solani infection ( Figure 2). The tested isolate expressed symptoms of pre-, post-emergence damping-off and root rot on all wheat cultivars. The highest pre-emergence damping-off values were observed on wheat cvs. Giza-171 (30%), Giza-168 and Misr-1 (28%). However, a low percentage of pre-emergence damping-off was observed on Sids-13 (15%). The percentages of postemergence damping-off varied from 33 to 40%. Giza-168, Giza-171, and Misr-2 were the most susceptible, which showed 40% post-emergence damping-off, while the lowest post- Figure 2. Pathogenicity of R. solani against eight Egyptian bread wheat cultivars. The experiment was repeated twice independently. Data presented are means ± standard deviation (mean ± SD) of five biological replicates.

In Vitro Antifungal Activity of SiO2 NPs on R. solani
The in vitro antifungal activity of biosynthesized SiO2 NPs was tested using two different methods ( Figure 3). SiO2 NPs showed a strong dose-dependent fungistatic activity against R. solani since the higher concentrations showed a wider inhibition zone and vice versa ( Figure 3A). The highest concentration of SiO2 (100 μg mL −1 ) showed no mycelial growth (100% growth reduction) of R. solani ( Figure 3A,B). Applying SiO2 NPs at the three concentrations (25, 50 and 100 μg mL −1 ) significantly reduced the linear growth of R. solani (y = −0.0762x + 6.56, R 2 = 0.7693; Figure 3C). Consequently, the inhibition (%) of the mycelial growth of R. solani was dose-dependent. No fungal growth was observed when mycelium was treated with 100 μg mL −1 SiO2 (100% growth reduction). Similarly, SiO2 NPs showed strong in vitro antifungal activity against R. solani growing on liquid media (Figure 3D) as expressed by inhibition of both mycelium fresh ( Figure 3E) and dry weight ( Figure 3F) of treated cultures. The highest concentration of SiO2 NPs (100 μg mL −1 ) was the most effective concentration in reducing the fresh and dry weight of R. solani mycelial growth by 91.0 and 93.5, respectively ( Figure 3E and Figure 3F, respectively).

In Vitro Antifungal Activity of SiO 2 NPs on R. solani
The in vitro antifungal activity of biosynthesized SiO 2 NPs was tested using two different methods ( Figure 3). SiO 2 NPs showed a strong dose-dependent fungistatic activity against R. solani since the higher concentrations showed a wider inhibition zone and vice versa ( Figure 3A). The highest concentration of SiO 2 (100 µg mL −1 ) showed no mycelial growth (100% growth reduction) of R. solani ( Figure 3A,B). Applying SiO 2 NPs at the three concentrations (25, 50 and 100 µg mL −1 ) significantly reduced the linear growth of R. solani (y = −0.0762x + 6.56, R 2 = 0.7693; Figure 3C). Consequently, the inhibition (%) of the mycelial growth of R. solani was dose-dependent. No fungal growth was observed when mycelium was treated with 100 µg mL −1 SiO 2 (100% growth reduction). Similarly, SiO 2 NPs showed strong in vitro antifungal activity against R. solani growing on liquid media ( Figure 3D) as expressed by inhibition of both mycelium fresh ( Figure 3E) and dry weight ( Figure 3F) of treated cultures. The highest concentration of SiO 2 NPs (100 µg mL −1 ) was the most effective concentration in reducing the fresh and dry weight of R. solani mycelial growth by 91.0 and 93.5, respectively ( Figure 3E and 3F, respectively).

SiO 2 NPs Increased the Extracellular Conductivity of Treated Fungal Suspension
Treating the mycelium of R. solani with SiO 2 NPs significantly increased levels of extracellular conductivity compared to control. The conductivity was increased progressively by the time of exposure with a greater effect with the highest concentration of SiO 2 NPs (100 µg mL −1 ). However, there was no significant effect between 12 and 24 h exposure time to the higher concentration of SiO 2 on the conductivity of the supernatant ( Figure 3G). . The experiments were repeated twice independently. In bar graphs, data presented are means ± standard deviation (mean ± SD) of five biological replicates. Different letters indicate statistically significant differences among treatments, while the same letters signify no significant differences between them according to Tukey's honestly significant difference test (p < 0.05). In simple linear regression graphs, the linear fit regression line is presented as a dotted line, regression equation and R 2 are also presented within the graph. . The experiments were repeated twice independently. In bar graphs, data presented are means ± standard deviation (mean ± SD) of five biological replicates. Different letters indicate statistically significant differences among treatments, while the same letters signify no significant differences between them according to Tukey's honestly significant difference test (p < 0.05). In simple linear regression graphs, the linear fit regression line is presented as a dotted line, regression equation and R 2 are also presented within the graph. Treating wheat grains with SiO 2 significantly increased the germinated grains compared with control ( Figure 4A). Infected and treated grains with SiO 2 NPs at 50 and 100 µg mL −1 showed a higher germination percentage compared with infected and nontreated seeds (positive control). The highest germination percentage 98% was observed in non-infected wheat seeds that were treated with SiO 2 NPs at a concentration of 100 µg mL −1 . No significant effect was found between the germination (%) of the negative control (untreated healthy seeds) and inoculated seeds that were treated with 100 µg mL −1 SiO 2 NPs ( Figure 4A). solani. Data presented are means ± standard deviation (mean ± SD) of five biological replicates. Different letters indicate statistically significant differences among treatments, while the same letters signify no significant differences between them according to Tukey's honestly significant difference test (p < 0.05). solani. Data presented are means ± standard deviation (mean ± SD) of five biological replicates. Different letters indicate statistically significant differences among treatments, while the same letters signify no significant differences between them according to Tukey's honestly significant difference test (p < 0.05).

SiO2 NPs Increased the Extracellular Conductivity of Treated Fungal Suspension
Likewise, SiO 2 NPs application significantly enhanced both root ( Figure 4B) and shoot lengths ( Figure 4C) of both healthy and R. solani-infected seedlings. As a result, all tested concentrations of SiO 2 NPs significantly increased the vigor index based on root and shoot length (SVIL; Figure 4D) in both healthy and infected wheat seedlings. Applying SiO 2 NPs at 50 and 100 µg mL −1 on healthy wheat seeds significantly increased SVIL values to 5552.9 and 5983.7, respectively. Additionally, treating infected wheat seeds with 50 and 100 µg mL −1 SiO 2 NPs resulted in SVIL values of 4419.6 and 4840.9, respectively, compared with 4413.4 for healthy untreated seedlings (negative control).
Similar results were observed in both seedling fresh weight ( Figure 4E), seedling dry weight ( Figure 4F), and when the seedling vigor index was measured based on seedling weight (SVIW; Figure 4G). The highest SVIW was noticed when healthy seeds were treated with 100 µg mL −1 SiO 2 NPs (284.4) followed by 50 µg mL −1 (224.4). All tested concentrations of SiO 2 NPs significantly increased SVIW of inoculated seedlings compared with negative and positive controls ( Figure 4G).

SiO 2 NPs Application Reduced the Disease Parameters of R. solani-Inoculated Wheat
Soil infestation with R. solani significantly elevated pre-, post-emergence damping-off, and root rot percentages on inoculated wheat seedlings. SiO 2 NPs application showed reduced disease frequency and completely protected wheat seedlings at 100 µg mL −1 ( Figure 5A). Untreated wheat seedlings grown in R. solani-infested soil showed 17.6% preemergence compared to 5.4% in untreated healthy seedlings ( Figure 5B). R. solani caused a significant increase in post-emergence damping-off and root rot ( Figure 5C,D) recording 32.2% and 38.4%, respectively, compared to 0% in the uninoculated negative control. In addition, treating the seeds with SiO 2 NPs significantly decreased the percentages of pre, post-emergence damping-off, and root rot compared to inoculated positive control. The highest concentration of SiO 2 NPs 100 µg mL −1 gave the lowest pre-emergence dampingoff (5%), post-emergence damping-off (5.2%), and root rot (8.4%), followed by SiO 2 NPs at 50 and 25 µg mL −1 .

SiO2 NPs Application Reduced the Disease Parameters of R. solani-Inoculated Wheat
Soil infestation with R. solani significantly elevated pre-, post-emergence dampingoff, and root rot percentages on inoculated wheat seedlings. SiO2 NPs application showed reduced disease frequency and completely protected wheat seedlings at 100 μg mL −1 (Figure 5A). Untreated wheat seedlings grown in R. solani-infested soil showed 17.6% preemergence compared to 5.4% in untreated healthy seedlings ( Figure 5B). R. solani caused a significant increase in post-emergence damping-off and root rot ( Figure 5C,D) recording 32.2% and 38.4%, respectively, compared to 0% in the uninoculated negative control. In addition, treating the seeds with SiO2 NPs significantly decreased the percentages of pre, post-emergence damping-off, and root rot compared to inoculated positive control. The highest concentration of SiO2 NPs 100 μg mL −1 gave the lowest pre-emergence dampingoff (5%), post-emergence damping-off (5.2%), and root rot (8.4%), followed by SiO2 NPs at 50 and 25 μg mL −1 .
. Figure 5. Effect of silicon dioxide nanoparticles (SiO2 NPs) on damping-off severity of wheat seedlings infected by R. solani. (A) Healthy (negative control), R. solani-infected (positive control), and SiO2-treated wheat seedlings, (B) pre-emergence damping-off, (C) Post-emergence damping-off, and (D) Root rot severity. Whiskers show the minimum and the maximum values, horizontal thick lines indicate the medians, boxes signify the interquartile ranges (25th to 75th percentile of the data). Different letters indicate statistically significant differences among treatments, while the same letters signify no significant differences between them according to Tukey's honestly significant difference test (p < 0.05; n = 5).  Different letters indicate statistically significant differences among treatments, while the same letters signify no significant differences between them according to Tukey's honestly significant difference test (p < 0.05; n = 5). Infection with R. solani adversely reduced the pigment content of infected wheat seedlings. In this regard, the chlorophyll a ( Figure 6A), chlorophyll b ( Figure 6B), and carotenoids ( Figure 6C) were reduced in the positive control (infected untreated seedlings) by 30, 30, and 20% relative to the negative control (untreated uninfected seedlings). On the other hand, the seedlings treated with SiO 2 NPS had a protective effect on wheat plants by alleviating the reduction of pigments contents higher than the healthy plants, which were witnessed at the level of 100 µg mL −1 . The positive effect of SiO 2 NPs was also reported on the healthy plants and the effect intensified as the concentration of SiO 2 NPs increased ( Figure 6). were witnessed at the level of 100 μg mL −1 . The positive effect of SiO2 NPs was also reported on the healthy plants and the effect intensified as the concentration of SiO2 NPs increased ( Figure 6). presented are means ± standard deviation (mean ± SD) of five biological replicates. Different letters indicate statistically significant differences among treatments, while the same letters signify no significant differences between them according to Tukey's honestly significant difference test (p < 0.05).

Treatment with SiO2 NPs Alleviated the Oxidative Stress in R. solani-Infected Plants
Infection with R. solani induced a high accumulation of hydrogen peroxide (129%; Figure 7A), superoxide anions (27%; Figure 7B), and hydroxyl radicals (17%; Figure 7C) compared with healthy plants (negative control). This effect was retarded by the applied levels of SiO2 NPS where the values of reactive oxygen species were lower than healthy plants ( Figure 7). Likewise, the results deduced that R. solani enhanced lipid peroxidation (56%; Figure 7D) and the contents of methylglyoxal (95%; Figure 7E) relative to healthy plants ( Figure 7). It is worthy to mention that applying SiO2 NPs with different concentrations decreased the peroxidation of lipids and methylglyoxal compared to pathogen-infected plants and the lowest reduction was recorded for the level of 100 μg mL −1 where lipid peroxidation and methylglyoxal increased only by 7.3 and 18.8% higher than healthy plants and decreased by 30% and 36.8% compared with the infected control, respectively ( Figure 7). Data presented are means ± standard deviation (mean ± SD) of five biological replicates. Different letters indicate statistically significant differences among treatments, while the same letters signify no significant differences between them according to Tukey's honestly significant difference test (p < 0.05).

Treatment with SiO 2 NPs Alleviated the Oxidative Stress in R. solani-Infected Plants
Infection with R. solani induced a high accumulation of hydrogen peroxide (129%; Figure 7A), superoxide anions (27%; Figure 7B), and hydroxyl radicals (17%; Figure 7C) compared with healthy plants (negative control). This effect was retarded by the applied levels of SiO 2 NPS where the values of reactive oxygen species were lower than healthy plants ( Figure 7). Likewise, the results deduced that R. solani enhanced lipid peroxidation (56%; Figure 7D) and the contents of methylglyoxal (95%; Figure 7E) relative to healthy plants ( Figure 7). It is worthy to mention that applying SiO 2 NPs with different concentrations decreased the peroxidation of lipids and methylglyoxal compared to pathogen-infected plants and the lowest reduction was recorded for the level of 100 µg mL −1 where lipid peroxidation and methylglyoxal increased only by 7.3 and 18.8% higher than healthy plants and decreased by 30% and 36.8% compared with the infected control, respectively ( Figure 7). ). Data presented are means ± standard deviation (mean ± SD) of five biological replicates. Different letters indicate statistically significant differences among treatments, while the same letters signify no significant differences between them according to Tukey's honestly significant difference test (p < 0.05).

SiO2 NPs Induced the Accumulation of Defense-Related Compounds in R. solani-Infected Seedlings
It is worth mentioning that the infection with R. solani significantly increased secondary metabolites and defense-related compounds. The infection increased the contents of total flavonoids ( Figure 8A) and total phenolics ( Figure 8B) by about 54 and 38%, respectively, relative to the healthy plants. However, the utilization of different levels of SiO2 NPs instigated the secondary metabolites in healthy and infected plants. The exposure of seedlings to 100 μg mL −1 had a prominent role relative to other levels for inducing secondary metabolites (Figure 8). At the same time, the application of SiO2 NPs significantly enhanced the accumulation of salicylic acid in infected seedlings, but not healthy ones (Figure 8C). The application of SiO2 NPs at the levels of 50 and 100 μg mL −1 elevated the reduction in SA content in infected plants to a higher level than in healthy plants. Moreover, the activity of phenylalanine ammonia-lyase (PAL; a key SA biosynthesis enzyme) was ). Data presented are means ± standard deviation (mean ± SD) of five biological replicates. Different letters indicate statistically significant differences among treatments, while the same letters signify no significant differences between them according to Tukey's honestly significant difference test (p < 0.05).

SiO 2 NPs Induced the Accumulation of Defense-Related Compounds in R. solani-Infected Seedlings
It is worth mentioning that the infection with R. solani significantly increased secondary metabolites and defense-related compounds. The infection increased the contents of total flavonoids ( Figure 8A) and total phenolics ( Figure 8B) by about 54 and 38%, respectively, relative to the healthy plants. However, the utilization of different levels of SiO 2 NPs instigated the secondary metabolites in healthy and infected plants. The exposure of seedlings to 100 µg mL −1 had a prominent role relative to other levels for inducing secondary metabolites (Figure 8). At the same time, the application of SiO 2 NPs significantly enhanced the accumulation of salicylic acid in infected seedlings, but not healthy ones ( Figure 8C). The application of SiO 2 NPs at the levels of 50 and 100 µg mL −1 elevated the reduction in SA content in infected plants to a higher level than in healthy plants. Moreover, the activity of phenylalanine ammonia-lyase (PAL; a key SA biosynthesis enzyme) was negatively affected by R. solani. The applied protectant increased the PAL activity, and the enhanced value was intensified as the concentration of SiO 2 NPs increased ( Figure 8D). negatively affected by R. solani. The applied protectant increased the PAL activity, and the enhanced value was intensified as the concentration of SiO2 NPs increased ( Figure 8D). a key SA biosynthesis enzyme) (μmol mg −1 protein). Data presented are means ± standard deviation (mean ± SD) of five biological replicates. Different letters indicate statistically significant differences among treatments, while the same letters signify no significant differences between them according to Tukey's honestly significant difference test (p < 0.05).

SiO2 NPs Stimulated the Non-Enzymatic Antioxidant Machinery of R. solani-Infected Seedlings
The non-enzymatic antioxidants, such as nitric oxide ( Figure 9A), ascorbic acid (vitamin C; Figure 9B), and glutathione (GSH; Figure 9C) were found at lower levels in nontreated R. solani-infected seedlings. However, these harmful effects were neutralized upon SiO2 NPs application ( Figure 9) in infected plants. For instance, nitric oxide (NO) recorded lower values for only R. solani-infected plants. The used applicants increased the NO content of wheat leaves compared to infected plants only ( Figure 9A). The highest induction was recorded also for the level of 100 μg mL −1 SiO2 NPs. Likewise, the pool of ascorbic acid content was significantly increased by the application of SiO NPs. Intriguingly, ascorbic acid recorded a high value under the interactive effect of 100 μg mL −1 SiO2 NPs and pathogen-infected plants compared with infected and nontreated control (positive control) ( Figure 9B). Similarly, reduced glutathione (GSH) in the infected plants seems to be deregulated by R. solani infection where the lowest values were obtained. The GSH levels were increased after the application of nanomaterial with high alleviation capacity at the concentration of 100 μg mL −1 SiO2 NPs ( Figure 9C). a key SA biosynthesis enzyme) (µmol mg −1 protein). Data presented are means ± standard deviation (mean ± SD) of five biological replicates. Different letters indicate statistically significant differences among treatments, while the same letters signify no significant differences between them according to Tukey's honestly significant difference test (p < 0.05).

SiO 2 NPs Stimulated the Non-Enzymatic Antioxidant Machinery of R. solani-Infected Seedlings
The non-enzymatic antioxidants, such as nitric oxide ( Figure 9A), ascorbic acid (vitamin C; Figure 9B), and glutathione (GSH; Figure 9C) were found at lower levels in nontreated R. solani-infected seedlings. However, these harmful effects were neutralized upon SiO 2 NPs application ( Figure 9) in infected plants. For instance, nitric oxide (NO) recorded lower values for only R. solani-infected plants. The used applicants increased the NO content of wheat leaves compared to infected plants only ( Figure 9A). The highest induction was recorded also for the level of 100 µg mL −1 SiO 2 NPs. Likewise, the pool of ascorbic acid content was significantly increased by the application of SiO NPs. Intriguingly, ascorbic acid recorded a high value under the interactive effect of 100 µg mL −1 SiO 2 NPs and pathogen-infected plants compared with infected and nontreated control (positive control) ( Figure 9B). Similarly, reduced glutathione (GSH) in the infected plants seems to be deregulated by R. solani infection where the lowest values were obtained. The GSH levels were increased after the application of nanomaterial with high alleviation capacity at the concentration of 100 µg mL −1 SiO 2 NPs ( Figure 9C). Plants 2021, 10, x FOR PEER REVIEW 12 of 26 Data presented are means ± standard deviation (mean ± SD) of five biological replicates. Different letters indicate statistically significant differences among treatments, while the same letters signify no significant differences between them according to Tukey's honestly significant difference test (p < 0.05).

SiO2 NPs Induced the Enzymatic Antioxidant Machinery of R. solani-Infected Seedlings
The antioxidant enzymes responded differentially to R. solani infection. SOD ( Figure  10A) and POD ( Figure 10B) activities were increased by 11 and 46%, respectively, relative to healthy plants. On the other hand, the activities of both APX ( Figure 10C) and CAT ( Figure 10D) were reduced by 21 and 10%, respectively, due to R. solani infestation. Nevertheless, the application of SiO2 NPs induced the antioxidant enzymes by restricting the reduction of APX and CAT and exacerbated the content of SOD compared to infected and healthy plants. It is worth mentioning that the activity of POD was kept at the level of infected plants under the interactive effect of SiO2 NPs and R. solani infection, but higher than control plants. The healthy plants treated with SiO2 NPs recorded higher activities of POD, APX and CAT compared to non-treated healthy plants. The activity of SOD in infected plants was kept at levels similar to the control irrespective of the level of SiO2 NPs applied ( Figure 10). Similarly, polyphenol oxidase (PPO) activity was found to be at the lowest content for healthy plants receiving no nano-silicon treatments ( Figure 10E). On the other hand, R. solani enhanced the PPO activity and the application of SiO2 NPs reduced PPO in infected plants compared with infected and nontreated control especially at the highest concentrations 100 μg mL −1 . presented are means ± standard deviation (mean ± SD) of five biological replicates. Different letters indicate statistically significant differences among treatments, while the same letters signify no significant differences between them according to Tukey's honestly significant difference test (p < 0.05).

SiO 2 NPs Induced the Enzymatic Antioxidant Machinery of R. solani-Infected Seedlings
The antioxidant enzymes responded differentially to R. solani infection. SOD ( Figure 10A) and POD ( Figure 10B) activities were increased by 11 and 46%, respectively, relative to healthy plants. On the other hand, the activities of both APX ( Figure 10C) and CAT ( Figure 10D) were reduced by 21 and 10%, respectively, due to R. solani infestation. Nevertheless, the application of SiO 2 NPs induced the antioxidant enzymes by restricting the reduction of APX and CAT and exacerbated the content of SOD compared to infected and healthy plants. It is worth mentioning that the activity of POD was kept at the level of infected plants under the interactive effect of SiO 2 NPs and R. solani infection, but higher than control plants. The healthy plants treated with SiO 2 NPs recorded higher activities of POD, APX and CAT compared to non-treated healthy plants. The activity of SOD in infected plants was kept at levels similar to the control irrespective of the level of SiO 2 NPs applied ( Figure 10). Similarly, polyphenol oxidase (PPO) activity was found to be at the lowest content for healthy plants receiving no nano-silicon treatments ( Figure 10E . Data presented are means ± standard deviation (mean ± SD) of five biological replicates. Different letters indicate statistically significant differences among treatments, while the same letters signify no significant differences between them according to Tukey's honestly significant difference test (p < 0.05).

Discussion
Spherical shaped nano silicon dioxide (SiO2) particles were successfully biosynthesized during this study using saffron extraction. The role of saffron in the biosynthesis of metal oxides nanoparticles was explained as the extract of saffron petals contains hydroxyl groups from several phenolic compounds, such as flavonoids like kaempferol and anthocyanins like anthocyanidin, delphinidin, and pelargonidin. These hydroxyl groups enhance saffron's ability for the biosynthesis of metal NPs, as it binds with metal ions and acts as a reducing agent for the reduction of metal crude particles to metal NPs [31,32]. It was previously inferred that biosynthesis of nanoparticles improves the physicochemical characteristics of particles, such as the surface area-to-volume ratio and enhances the stability of the structure that improves the anti-microbial activity of the nanometals against plant pathogens.
In this study, SiO2 NPs were biosynthesized using saffron extract. The maximum peak of SiO2 NPs was observed at approximately 440 nm, which is almost the same finding . Data presented are means ± standard deviation (mean ± SD) of five biological replicates. Different letters indicate statistically significant differences among treatments, while the same letters signify no significant differences between them according to Tukey's honestly significant difference test (p < 0.05).

Discussion
Spherical shaped nano silicon dioxide (SiO 2 ) particles were successfully biosynthesized during this study using saffron extraction. The role of saffron in the biosynthesis of metal oxides nanoparticles was explained as the extract of saffron petals contains hydroxyl groups from several phenolic compounds, such as flavonoids like kaempferol and anthocyanins like anthocyanidin, delphinidin, and pelargonidin. These hydroxyl groups enhance saffron's ability for the biosynthesis of metal NPs, as it binds with metal ions and acts as a reducing agent for the reduction of metal crude particles to metal NPs [31,32]. It was previously inferred that biosynthesis of nanoparticles improves the physicochemical characteristics of particles, such as the surface area-to-volume ratio and enhances the stability of the structure that improves the anti-microbial activity of the nanometals against plant pathogens.
In this study, SiO 2 NPs were biosynthesized using saffron extract. The maximum peak of SiO 2 NPs was observed at approximately 440 nm, which is almost the same finding as reported by Tripathi et al. [33]. FTIR spectroscopy uses wavelength to measure the absorption of infrared radiation by tested samples, the reading of the infrared spectrum includes the interpretation of the correlation between the absorption bands (vibration bands) and the chemical compounds in the sample. The spectra of SiO 2 NPs showed a band around 1103 cm −1 which corresponds to the asymmetric stretching vibration of Si-O-Si [34][35][36]. A wide absorption range was observed at 1634 and 3405 cm −1 that indicates the presence of H-O-H stretching and bending of absorbed water [37,38]. The observed peaks at 801 cm −1 are assigned to the Si-OH bond [34,36].
The broadband detected with XRD which showed reflection at 2 as reported by Tripathi et al. [33]. FTIR spectroscopy uses wavelength to measure the absorption of infrared radiation by tested samples, the reading of the infrared spectrum includes the interpretation of the correlation between the absorption bands (vibration bands) and the chemical compounds in the sample. The spectra of SiO2 NPs showed a band around 1103 cm −1 which corresponds to the asymmetric stretching vibration of Si-O-Si [34][35][36]. A wide absorption range was observed at 1634 and 3405 cm −1 that indicates the presence of H-O-H stretching and bending of absorbed water [37,38]. The observed peaks at 801 cm −1 are assigned to the Si-OH bond [34,36]. The broadband detected with XRD which showed reflection at 2Ѳ = 22.8 o and the strong absorption band at 440 nm by UV-vis indicated that amorphous SiO2 nanoparticles were successfully synthesized [33,39]. Additionally, no additional peaks were observed in the XRD spectrum which indicates there are no impurities in the obtained SiO2 NPs. Additionally, the percentage of each element was calculated using the energy dispersion spectrum (EDS) which showed that SiO2 NPs contained 29% Si and 71% O. SiO2 NPs sized between 20 and 95 nm were synthesized by sol-gel method using sodium silicate [33]. According to UV-Vis, FTIR, XRD, and TEM images, using saffron extraction in the biosynthesis of SiO2 NPs resulted in smaller particle sizes 9.92 to 19.8 nm with safer and fewer coast methods.
The importance of SiO2 NPs lays in their dual effect on both pathogen and host plant. On the pathogen side, silicon dioxide nanoparticles showed high antifungal activity against R. solani and completely inhibited its growth at 100 μg mL −1 . The antifungal effect of SiO2 NPs against the human pathogenic Trichoderma Harzianum and Rhizoctonia species was previously reported by Verma and Bhattacharya [35]. Moreover, Derbalah et al. stated that SiO2 NPs showed an antifungal effect against Alternaria solani, which significantly inhibited the growth of Alternaria mycelium and reduced the severity of early blight disease on tomato plants [40].
Various theories explained the fungicidal effect of silicon nanoparticles. The accumulation of SiO2 NPs in the membrane of the fungal cell wall may result in the lysis of the cells, blockage of the transmembrane energy cycle, disruption of the electron transport chain, or oxidation of the cell membrane by forming insoluble compounds in the cell membrane. SiO2 NPs interact with protein thiol groups (-SH) on the fungal cell surface leading to cell lysis due to its positive charge [40]. Silicon nanoparticles may deactivate the protein molecules and directly bind with fungal DNA causing mutation and affecting replication [41]. Furthermore, hydroxyl groups on the surface of small particles of silicon bind with lipopolysaccharides of the fungal cell wall and cause a breakdown of treated fungal cells [42]. In this study, the loss of integrity of R. solani cell wall and cell membrane was confirmed by leakage of cellular materials, which resulted in changes in extracellular conductivity.
On the host plant side, It is well-documented that silicon application positively increases the host plant resistance against phytopathogens and plays important role in the interaction between the host plant and the pathogen [43]. Additionally, it decreases the severity of fungal diseases and induced resistance against a wide range of plant pathogenic fungi that cause root and foliar diseases [25,44]. It is worth mentioning that biosynthesized SiO2 NPs showed decreased pre-, post-emergence damping-off and root rot percentages of infected wheat seedlings in the current study. This might be due to the negative effects of SiO2 NPs on the fungal pathogen since our findings showed a strong dosedependent fungistatic activity against R. solani in vitro. For instance, the highest concentration of SiO2 (100 μg mL −1 ) showed no mycelial growth (100% growth reduction) of R. solani.
Moreover, the suppression of pre-, post-emergence damping-off and root rot severity caused by SiO2 NPs could be attributed to its contribution to different defense mechanisms. One of the defense mechanisms that could be expressed by silicon is the formation of physical barriers through Si accumulation below the cuticle and in cell walls, which = 22.8 o and the strong absorption band at 440 nm by UV-vis indicated that amorphous SiO 2 nanoparticles were successfully synthesized [33,39]. Additionally, no additional peaks were observed in the XRD spectrum which indicates there are no impurities in the obtained SiO 2 NPs. Additionally, the percentage of each element was calculated using the energy dispersion spectrum (EDS) which showed that SiO 2 NPs contained 29% Si and 71% O. SiO 2 NPs sized between 20 and 95 nm were synthesized by sol-gel method using sodium silicate [33]. According to UV-Vis, FTIR, XRD, and TEM images, using saffron extraction in the biosynthesis of SiO 2 NPs resulted in smaller particle sizes 9.92 to 19.8 nm with safer and fewer coast methods.
The importance of SiO 2 NPs lays in their dual effect on both pathogen and host plant. On the pathogen side, silicon dioxide nanoparticles showed high antifungal activity against R. solani and completely inhibited its growth at 100 µg mL −1 . The antifungal effect of SiO 2 NPs against the human pathogenic Trichoderma Harzianum and Rhizoctonia species was previously reported by Verma and Bhattacharya [35]. Moreover, Derbalah et al. stated that SiO 2 NPs showed an antifungal effect against Alternaria solani, which significantly inhibited the growth of Alternaria mycelium and reduced the severity of early blight disease on tomato plants [40].
Various theories explained the fungicidal effect of silicon nanoparticles. The accumulation of SiO 2 NPs in the membrane of the fungal cell wall may result in the lysis of the cells, blockage of the transmembrane energy cycle, disruption of the electron transport chain, or oxidation of the cell membrane by forming insoluble compounds in the cell membrane. SiO 2 NPs interact with protein thiol groups (-SH) on the fungal cell surface leading to cell lysis due to its positive charge [40]. Silicon nanoparticles may deactivate the protein molecules and directly bind with fungal DNA causing mutation and affecting replication [41]. Furthermore, hydroxyl groups on the surface of small particles of silicon bind with lipopolysaccharides of the fungal cell wall and cause a breakdown of treated fungal cells [42]. In this study, the loss of integrity of R. solani cell wall and cell membrane was confirmed by leakage of cellular materials, which resulted in changes in extracellular conductivity.
On the host plant side, It is well-documented that silicon application positively increases the host plant resistance against phytopathogens and plays important role in the interaction between the host plant and the pathogen [43]. Additionally, it decreases the severity of fungal diseases and induced resistance against a wide range of plant pathogenic fungi that cause root and foliar diseases [25,44]. It is worth mentioning that biosynthesized SiO 2 NPs showed decreased pre-, post-emergence damping-off and root rot percentages of infected wheat seedlings in the current study. This might be due to the negative effects of SiO 2 NPs on the fungal pathogen since our findings showed a strong dose-dependent fungistatic activity against R. solani in vitro. For instance, the highest concentration of SiO 2 (100 µg mL −1 ) showed no mycelial growth (100% growth reduction) of R. solani.
Moreover, the suppression of pre-, post-emergence damping-off and root rot severity caused by SiO 2 NPs could be attributed to its contribution to different defense mechanisms. One of the defense mechanisms that could be expressed by silicon is the formation of physical barriers through Si accumulation below the cuticle and in cell walls, which contributed to preventing or delaying the penetration of infection pegs of R. solani appressoria [45,46]. Additionally, silicon effectively prevents fungal ingress by the formation of a Si-enriched layer and the uniform distribution of Si aggregates [43,44].
The accurate biological mechanisms of potential interaction between silicon and different biochemical pathways that lead to plant resistance to fungal pathogens remain unclear [46]. The defense mechanisms induced by silicon involve rapid production of defense compounds, i.e., phenolics, flavonoids, anthocyanins, lignin, callose, and phytoalexins through primary, as well as secondary metabolic pathways, also silicon increased activities of defense enzymes, such as phenylalanine ammonia-lyase (PAL), polyphenol oxidase (PPO), peroxidase (POX), lipoxygenase (LOX), chalcone synthase (CHS) chalcone isomerase, β-1,3-glucanase (GLU), pathogenesis-related (PR) proteins and chitinases [47][48][49]. Interestingly, our findings showed that SiO 2 NPs application simultaneously activated multiple defense mechanisms in treated wheat seedlings. These mechanisms involve (i) the induction of defense-related compounds, particularly SA accumulation and its major biosynthetic enzyme PAL, and (ii) activation of both enzymatic (POD, SOD, APX, CAT, and PPO) and non-enzymatic (phenolics and flavonoids) antioxidant defense machinery.
In addition, the alteration of membrane phospholipids acts as signaling components during R. solani infection. In the current study, the infected plants suffered from high damage of the membrane by exacerbation of lipid peroxidation content, which was repeatedly outlined in the literature as an indicator of the oxidative burst in stressed plants [50]. Methylglyoxal (MG) accumulation was shown to be correlated with increased intracellular oxidative stress, due to enhanced reactive oxygen species (ROS) production [50]. The studied plants encountered a high accumulation of MG content under R. solani infection.
The excessive MG accumulation in plant cells under infection by R. solani can inhibit cell proliferation, chlorophyll biosynthesis, instigate the deactivation and/or degradation of proteins, as well as antioxidant defending products, leading to disruption of many cellular functions [51]. All these deteriorations induced by R. solani were augmented by SiO 2 NPS. The SiO 2 NPs upregulated the content of MG and lipid peroxidation concomitant with reduction of ROS and augmentation of antioxidants and chlorophyll content. Thus, SiO 2 NPs triggered better intact membrane structure through the reduction of the fluid structure of membrane lipids. The situation was confirmed by lower ROS, lipid peroxidation, and methylglyoxal activity. Thus, wheat plants respond to nanoparticles by fine-tuning redox homeostasis and so resist R. solani infection. Si and Si nanoparticles might play an important role in promoting protective mechanisms to decline membrane lipid peroxidation and electrolyte leakage through NO-signaling [33].
Moreover, the interaction between salicylic acid (SA) and reactive oxygen species (ROS) is well-documented [52]. The SA-ROS plays a key role in the transcriptional reprogramming that occurs during the plant defense responses. Briefly, biotic stress, such as exposure to phytopathogenic fungi, triggers ROS production mainly at the apoplast [52]. As a result, plants try to defend themselves via multilayered defense mechanisms in a spatio-temporal manner via an SA-mediated pathway [52]. It is worth mentioning that SA not only has a pro-oxidant role, but it also plays an antioxidant role concertedly with glutathione (GSH) [52]. Interestingly, our findings showed that while infection with R. solani induced a high accumulation of hydrogen peroxide, superoxide anions, and hydroxyl radical compared with healthy plants, SiO 2 NPs application reduced the ROS levels and induced the accumulation of defense-related compounds, particularly SA, in R. solani-infected seedlings. Collectively, these findings suggest that SiO 2 NPs application might activate a feed-forward loop between ROS and SA in response to pathogen infection. However, further studies are required to better understand the molecular mechanisms of SiO 2 NPs in the stimulation of SA-ROS interplay.
Furthermore, the utilization of SiO 2 NPs had a regulatory role in stimulating the biosynthesis of ascorbate as an antioxidant molecule that keeps ROS (superoxide anion, hydrogen peroxide, and hydroxyl radical) at lower levels than the infected plants in a concentration-dependent manner where 100 mg L −1 was the most effective concentration. Similarly, our findings showed that R. solani infection shifted the cellular redox balance toward a more oxidative state, including a decline of the GSH pool, affecting all cellular compartments, and ROS detoxification. A similar reduction was reported for onion under Fusarium oxysporum infection [53].
Moreover, our findings showed that although R. solani significantly stimulated the content of the superoxide anions, the activity of SOD was enhanced upon SiO 2 NPs application. On the other hand, the high accumulation of H 2 O 2 was ascribed to the reduction of CAT and APX activities in non-treated infected plants, suggesting the sensitivity of the studied plants to infection by R. solani and breakdown of main defense strategies, which weaken the resistance of plants. However, SiO 2 NPs application significantly induced the activities of SOD, CAT, and APX in connection with the reduction of disease severity, ROS, and membrane deterioration traits (lipid peroxidation and methyloxyal). Furthermore, enhanced antioxidant enzymes activities played a key regulatory role in plant growth, photosynthetic rate, cellular redox potential, and membrane integrity by eliminating free radicals [54]. Our findings showed that Si NPs significantly improved activities of SOD, APX, CAT, and GPX, which further counterbalance ROS as indicated by lower lipid peroxidation and electrolyte leakage [33]. Collectively, our findings indicate that SiO 2 NPs enhance the wheat defense response against R. solani via upregulation of both enzymatic and non-enzymatic antioxidant defense machinery.
Apart from their role in catalyzing the breakdown of H 2 O 2 , PODs were reported to be involved in lignification and suberization processes [55]. POD activity of all SiO 2 NPs-treated plants under stress was lower than that of the control levels. Decreased activity of POD revealed that using SiO 2 NPs might reduce lignification processes resulting from R. solani infection. Therefore, SiO 2 NPs can reduce stress severity where there is no need for high lignification as reported by Bagy et al. [55] who reported that mycorrhizal fungi and entophyte reduce the content of soluble and ionic peroxidases and lignification under Pectobacterium infection.
In the present study, R. solani stimulated the production of phenolic compounds of wheat plants compared to healthy plants concomitant with enhanced peroxidase activity. Thus, the accumulation of phenolic compounds is a positive sign of stimulation of resistance by SiO 2 NPs, which significantly exacerbated phenolic compound production higher than in infected plants. Using nano-silica increased the contents of phenolics similar to the studies of [56,57]. Moreover, SiO 2 NPs application significantly induced the accumulation of defense-related compounds in R. solani-infected seedlings, particularly SA. SA is a defense-associated phytohormone that is mainly involved in plant responses to biotrophic and necrotrophic pathogens [58][59][60][61]. Furthermore, the major SA-biosynthetic enzyme, PAL, was dramatically reduced by infection; however, SiO 2 NPs promptly augmented the reduction of PAL under stress and further enhanced the activity of PAL, which is concomitant with the high induction of phenolic compounds and flavonoids. PAL is involved in the synthesis of plant secondary antimicrobial substances and it is essential for plant disease resistance responses [53] and plays an essential role in the biosynthesis of the precursors of lignin [62].
Plant defense via lignification is a conserved basal mechanism in the plant immune response against pathogens [63]. Silicon increases the transcript abundance of PAL in rice plants, leading to enhanced lignification [64], while SiO 2 NPs enhance PAL expression and lignification in the leaves and roots of oat seedlings [65]. The reduction of disease severity in rice [66] and cucumber [67] by silicon pre-treatment has been attributed to an increase in the activities of PPO and PAL. Therefore, the increase in the activity of PPO and PAL in the present study could prevent the pathogenic infection in beetroot due to silicon supplementation.
PPO activity was significantly stimulated upon treatment with SiO 2 NPs during fungal infection compared with healthy plants. This role of SiO 2 NPs revealed that the SiO 2 NPs reduced the pathogenesis, so the need for higher PPO in infected plants is not needed. PPO is a defense enzyme associated with fostering host resistance because it can catalyze the final step of lignin biosynthesis [62], and oxidize phenolic compounds to quinones [55]. The resulting quinones are toxic to invading organisms [68], hence possessing antipathogenic properties [69]. Consequently, SiO 2 NPs treatment reduces the severity of invading microorganisms and enhances suitable defending agents that support plant immunity. POD, PPO, and PAL defense enzymes are generally working together for enhancing plant resistance to pathogens. This conclusion was recommended for infected plants treated with SiO 2 NPs that had adequate PPO and PAL activities, which aided in preventing further development of infection.

Preparation of Aqueous Saffron Extraction
The aqueous saffron extraction was prepared as described by Nagaonkar et al. [70] with slight modification. Briefly, one gram of dried saffron stigmas (Qingdao Jingtai Huacheng International Trad Co., Ltd., Qingdao, Shandong, China) was suspended in 100 mL of deionized water. The mixture was homogenized and kept at 60 • C for 6 h. The obtained extract was filtered three times using Whatman filter paper no. 1 and further used in the process of synthesis of SiO 2 NPs.

Synthesis of SiO 2 Nanoparticles
SiO 2 NPs were prepared following the protocols described previously [71][72][73] with slight modifications. Briefly, 100 mL of the aqueous saffron extract was mixed with 100 mL of 0.1 M bulk SiO 2 (Qingdao Jingtai Huacheng International Trad Co., Ltd. Model No. XR.16, Silicon Dioxide) solution. The prepared solution was stirred at 60 • C for 6 h, then centrifuged at 10,000 rpm for 10 min. The supernatant was discarded and the pellets were collected and lyophilized to obtain the powder.

Characterization of SiO 2 Nanoparticles Analysis of Ultraviolet Spectra
SiO 2 NPs were checked at a wavelength ranging from 200 to 800 nm for the highest peak absorption using UV-Vis spectroscopy (Shimadzu Spectrometer, Shimadzu Corporation, Kyoto, Japan) [74].

Fourier Transform Infrared Spectroscopy (FTIR)
Formation of SiO 2 NPs was detected in the collected powder using FTIR analysis at a range of 400-4000 cm −1 regions using Fourier transform infrared spectrometer (Vector 22, Bruker, Germany) at a resolution of 4 cm −1 .

X-ray Diffraction (XRD)
The purity of extracted particles was tested using an X-ray diffractometer (XRD) by fixing a coated film of dried SiO 2 NPs powder on glass slides with operating conditions of 45 kV and 20 mA current with Cu-Ka radiation as an X-ray source in the 20-80 • range at the 2 14 of 26 [33]. FTIR spectroscopy uses wavelength to measure the abby tested samples, the reading of the infrared spectrum inthe correlation between the absorption bands (vibration pounds in the sample. The spectra of SiO2 NPs showed a corresponds to the asymmetric stretching vibration of Si-Orange was observed at 1634 and 3405 cm −1 that indicates the and bending of absorbed water [37,38]. The observed peaks Si-OH bond [34,36]. with XRD which showed reflection at 2Ѳ = 22.8 o and the nm by UV-vis indicated that amorphous SiO2 nanoparticles d [33,39]. Additionally, no additional peaks were observed indicates there are no impurities in the obtained SiO2 NPs. of each element was calculated using the energy dispersion d that SiO2 NPs contained 29% Si and 71% O. SiO2 NPs sized synthesized by sol-gel method using sodium silicate [33]. XRD, and TEM images, using saffron extraction in the bioin smaller particle sizes 9.92 to 19.8 nm with safer and fewer Ps lays in their dual effect on both pathogen and host plant. n dioxide nanoparticles showed high antifungal activity ely inhibited its growth at 100 μg mL −1 . The antifungal effect n pathogenic Trichoderma Harzianum and Rhizoctonia species Verma and Bhattacharya [35]. Moreover, Derbalah et al. an antifungal effect against Alternaria solani, which signifiof Alternaria mycelium and reduced the severity of early ts [40]. angle.

Transmission Electron Microscopy (TEM)
The transmission electron microscope JEM-1230, JEOL, Akishima, Japan, was used to detect the morphology of SiO 2 nanoparticles. The samples were processed as described by Atallah et al. [75]. A film from the sample was placed in a grid box and the procedures recommended by the manufacturer were followed.

Pathogen Isolate and Pathogenicity Test
An isolate of R. solani was obtained from the Department of Plant Pathology, Minia University, Egypt. The isolate was previously identified at Molecular Biology Research Unit, Assiut University and SolGent Company, Daejeon South Kore based on sequence analysis of the internal transcribed spacer (ITS) region using ITS1 and ITS4 primers. The R. solani isolate was propagated on a PDA medium, incubated for seven days at room temperature (28 ± 2 • C), and used as an inoculum source for the inoculation of wheat seeds [76,77].
The pathogenicity of R. solani isolate was tested on eight wheat cultivars namely Gemmiza-11, Gemmiza-12, Giza-168, Giza-171, Misr-1, Misr-2, Sids-13, and Sids-14. Briefly, sterilized soil was added to three-inches diameter pots. The inoculum of R. solani was cultured on barley grains was mixed with the soil at 1% (W: W). The infested pots were watered as needed and left for five days to enhance the establishment of R. solani growth in the soil. 1% sodium hypochlorite solution was used to surface sterilize the seeds of each wheat cultivar by immersing the seeds for 2 min in the solution. The seeds were then rinsed in sterile distilled water. Three seeds were sown in each pot. Five replicates were used for each treatment. Pots filled with non-infested soil were used as a negative control. The pots were randomly distributed within each plot. Pre-, post-emergence damping-off and root rot for wheat seedlings were evaluated two, four, and six weeks after the sowing date, respectively, according to Raju and Naik [78] and Beale et al. [79].
The pre-and post-emergence damping-off was calculated using Equation (1) as follows: Furthermore, the disease severity of root rot was assessed using the indexing method described by Beale et al. [79]. The roots of wheat plants were washed and divided into five categories according to the percentage of all roots with lesions typical of root rot: zero (0) trace to 10% (1), >10% and ≤30% (2), >30% and ≤60% (3), and >60% (4). Disease severity percentage was calculated using Equation (2)  The experiment was implemented as described by Joshi et al. [80] with minor modifications. Potato dextrose agar (PDA) medium was prepared, and SiO 2 NPs were amended into the media to obtain a final concentration of 25, 50, and 100 µg mL −1 . The media was poured into 9 cm diameter Petri dishes. After solidification, a 0.5 cm diameter disc of 5 days old R. solani culture was placed at the center of the dishes. The reduction percentage of pathogen growth was calculated using Equation (3) [81,82] as follows: Inhibition of pathogen growth (%) = growth in the control − growth in the treatment growth in the control × 100

Effect of SiO 2 NPs on the Mycelium Fresh and Dry Weight of R. solani
Mycelium dry weight was assessed according to the method described by Li et al. [83] with minor modifications. 50 mL of potato dextrose broth (PDB) medium was poured into a 250 mL Erlenmeyer flask. SiO 2 NPs were added to the media and the concentration was adjusted to 25, 50, and 100 µg mL −1 . No SiO 2 NPs were added to the control; 0.5 cm diameter disc of 5 days old R. solani culture was placed gently on the surface of PDB media. The inoculated flasks were incubated at 28 ± 2 • C for 5 days. For fresh weight assessment, the mycelium of R. solani from liquid media was harvested using a filtration-based method as previously described by Newell and Statzell-Tallman [84] with slight modifications. Briefly, the fungal mycelium was filtrated using a 40-µm-mesh nylon screen, washed with 25 mL distilled water, recollected on Whatman filter paper no. 1, then vacuumed for 30 s to abandon any free water from the samples. Subsequently, mycelia were kept in small Petri dishes to avoid rapid dehydration during fresh-weighting [84]. Fresh weight was assessed immediately after filtration. Samples were processed one by one through filtration and fresh-weighting. For dry weight assessment, the mycelia of R. solani left to dry at 50 • C for 24 h and reweighted. During the dry weight assay, fresh desiccant was maintained in the weighting chamber of the balance. The percentage of mycelium fresh and dry growth reduction was calculated according to Equation (4) as follows: Inhibition of mycelium fresh/dry weight (%) = Mycelium fresh/dry weight of control − Mycelium fresh/dry weight in the treatment Mycelium fresh/dry weight of control × 100 Five replicates were used for each concentration each replicate was represented with one flask. The experiment was repeated twice.

Extracellular Conductivity
Extracellular conductivity assay was carried out using a method described by Mahas and Kaur [85] with minor modifications. To obtain the fungal mycelium, 50 mL of nutrient broth (NB) was inoculated by a 6 mm mycelial disk of five days old R. solani culture. The inoculated NB was incubated for three days at 26 • C. Sterile distilled water was used to wash the collected mycelium. 100 mg of collected mycelium was transferred into 50 mL PDB containing three concentrations of 25, 50, and 100 µg mL −1 of SiO 2 NPs, and no particles were added to the control. The supernatants were collected at 0, 12, and 24 h of incubation by centrifuging the mycelial suspensions for 10 min at 10,000 rpm. The electrical conductivity of the supernatants was measured using a conductivity meter.

Effect of SiO 2 NPs on Germination, Root and Shoot Length, and Vigor Indexes of R. solani-Infected Wheat Seedlings
This experiment was conducted to study the effect of three SiO 2 NPs concentrations, 25, 50, and 100 µg mL −1 , on the germination percentage, root length, shoot length, and vigor index of wheat cv. Misr-2 infected with R. solani. Inoculation with fungal isolate was the main plot, and SiO 2 NPs treatment was the subplot. Five replicates were used for each treatment; three wheat seeds were sown in each pot as one replicate. The seeds of wheat cultivar Misr-2 were soaked in three concentrations of SiO 2 NPs, 25, 50, and 100 µg mL −1 for 12 hr. The seeds were then divided into two groups; the first group was sown in 15 pots, which were previously inoculated with R. solani as described in the cultivar evaluation test. Five pots were used for each concentration of SiO 2 NPs. The second group was sown in the same way except the soil was not inoculated with R. solani. Two controls were used in this experiment; Negative control (wheat seeds were soaked in water and sown in non-inoculated soil), Positive control (wheat seeds were soaked in water and sown in inoculated soil).
Two weeks after sowing dates, the wheat seedling was taken out of the pots and the roots were gently washed. The percentage of germinated seeds, roots, and shoots length, fresh and dry weight of wheat seedlings were measured. The germination percentage was calculated using Equation (5): Number of germinated seeds Number of total seeds × 100 Moreover, the vigor index of wheat seedlings was calculated using two traits. Seedling vigor index based on the root and shoot length (SVIL) was measured according to Equation (6) as described by Abdul-Baki and Anderson [16] as follows: SVIL = (shoot length + root length) × germination (%) (6) Likewise, the seedling vigor index based on the weight was calculated using Equation (7) as follows: SVIW = seedling dry mass at the end of the test × germination (%) (7) 4.5. Effect of SiO 2 on Pre-and Post-Emergence Damping-Off and Root Rot of Wheat under Inoculation with R. solani Wheat cultivar Misr-2 was used for this test. Wheat seeds were treated with SiO 2 NPs at three concentrations, 25, 50, and 100 µg mL −1 for 12 h. The treatments and experiment design were implemented as described in the above section. The inoculation was done as described in the cultivar evaluation test section. Pre-, post-emergence damping-off and root rot for wheat seedlings were evaluated two, four, and six weeks after the sowing date, respectively, as described previously.

Stress-Associated Biochemical and Physiological Assessments
The experiment was conducted and designed in the same way as described in the vigor index section. Leaves of three weeks old wheat seedlings from each treatment were used for the following measurements and five biological replicates were used for each trait.

Pigments Content
Chlorophyll a, b and carotenoids were measured in fresh leaves (0.05 g) suspended in 5 mL of ethyl alcohol (95%) using equations recommended by Lichtenthaler [86].

Membrane Damage Criteria
Lipid peroxidation was detected as described by Madhava Rao and Sresty [90] with some modifications. The thiobarbituric acid reaction was used to determine lipid peroxidation in wheat shoots by monitoring malondialdehyde formation as explained Methylglyoxal (MG) was estimated based on the method of Gilbert and Brandt [91].

Resistance-Related Compounds and Enzymes Salicylic Acid (SA)
Fresh wheat leaves were used for the determination of SA as described by Warrier et al. [92]. Briefly, 100 mg of leaf tissue were ground to a fine powder using liquid nitrogen, extracted with 1.0 mL of extraction solvent (chloroform, amyl alcohol, ether, and ethanol), then centrifuged at 10,000× g for 10 min. subsequently, 100 µL of the supernatant with up to 3 mL of freshly prepared ferric chloride (0.1%) till the development of violet color. The absorbance of the complex was measured using spectrophotometry at 540 nm [92].

Phenolic Compounds
Phenolic compounds were determined using a Folin-Ciocalteu-based method as described by Kofalvi and Nassuth [93], using gallic acid as a standard curve. Total phenolics were expressed as mg g −1 FW. Briefly, 300 mg fresh leaf tissues were extracted in methanol (50%) in a water bath (70 • C) for one hour. The methanolic extract was mixed with distilled water + Folin-Ciocalteu's reagent + Na 2 CO 3 at room temperature. After 20 min, the absorbance spectrum was measured at 725 nm.

Nitric Oxide Content (NO)
Nitric oxide (NO) content was indirectly determined as described by Ding et al. [94] and modified by Hu et al. [95]. Briefly, NO was reacted with Greiss reagent (l% sulfanil-amide/0.1% N-(l-naphthyl)-ethylenediamine dihydrochloride in 5% phosphate acid) was added for 30 min at room temperature till the appearance of azo violet color, which was measured spectrophotometrically at 550 nm. NaNO 2 was used to prepare the standard curve and the NO content was expressed as nmol g −1 FW.

Flavonoids Content
Total flavonoid content was colorimetrically assessed as described by Zou et al. [98] using aluminum chloride with slight modifications. Briefly, 100 mg of leaf tissue was ground to a fine powder using liquid nitrogen, extracted with 1.0 mL methanol, then centrifuged at 10,000× g for 10 min. Subsequently, about 0.5 mL of the supernatant was mixed with 2 mL of distilled water and 150 µL of 5% sodium nitrate and incubated for 6 min. After incubation, 150 µL of aluminum chloride (10%) and 2 mL of sodium hydroxide (1 M) were added and re-incubated at room temperature for 15 min. The absorbance of the mixtures was measured at 510 nm.

Statistical Analysis
Throughout this study, all experiments were laid out using a full factorial split-plot design arranged in completely randomized blocks using R. solani-infection (healthy vs. infected) as main plots and SiO 2 treatments (0, 25, 50, and 100 µg mL −1 SiO 2 ) in the subplots. All experiments were carried out using at least three biological replicates for each treatment. The analysis of variance (ANOVA) was used to test the significant differences among different infection levels (p infection ), treatments (p treatment ), and their interaction (p infection×treatment ). Tukey's honestly significant difference (HSD) test was used for posthoc analysis (p infection×treatment < 0.05). The data were analyzed using JMP data analysis software version 14.

Conclusions
In conclusion, SiO 2 NPs treatment reduced the infection rate and suppressed the growth of R. solani on wheat. Our findings demonstrated that SiO 2 NPs mitigate the negative effect of R. solani on wheat seedlings via the simultaneous activation of a multilayered defense system that involves at least three key mechanisms. (i) SiO 2 NPs have a direct dose-dependent fungistatic activity against the vegetative growth of R. solani. (ii) SiO 2 NPs induced the accumulation of defense-related compounds, particularly SA and its major biosynthetic enzyme PAL, and (iii) SiO 2 NPs induce the activation of both enzymatic (POD, SOD, APX, CAT, and PPO) and non-enzymatic (phenolics and flavonoids) antioxidant defense machinery to neutralize the destructive effect of ROS, lipid peroxidation, and methylglyoxal to maintain their homeostasis within R. solani-infected plants. Collectively, it is plausible to propose that the application of SiO 2 NPs could be considered as an alternative/eco-friendly approach to protect wheat plants from root rot-causing phytopathogenic fungi due to their suppressive role against the infection caused by R. solani.

Institutional Review Board Statement: Not applicable.
Informed Consent Statement: Not applicable.

Data Availability Statement:
The data that supports the findings of this study are contained within the article or Supplementary Materials and available from the corresponding author upon reasonable request.