Effects of Arbuscular Mycorrhizal Fungi on the Growth and Root Cell Ultrastructure of Eucalyptus grandis under Cadmium Stress

Eucalyptus grandis (E. grandis) has been reported to form a symbiosis with arbuscular mycorrhizal fungi (AMF), which plays an important role in improving plant tolerance of heavy metal. However, the mechanism of how AMF intercept and transport cadmium (Cd) at the subcellular level in E. grandis still remains to be researched. In this study, a pot experiment was conducted to investigate the growth performance of E. grandis under Cd stress and Cd absorption resistance of AMF and explored the Cd localization in the root by using transmission electron microscopy and energy dispersive X-ray spectroscopy. The results showed that AMF colonization could enhance plant growth and photosynthetic efficiency of E. grandis and reduce the translocation factor of Cd under Cd stress. After being treated with 50, 150, 300, and 500 μM Cd, the translocation factor of Cd in E. grandis with AMF colonization decreased by 56.41%, 62.89%, 66.67%, and 42.79%, respectively. However, the mycorrhizal efficiency was significant only at low Cd concentrations (50, 150, and 300 μM). Under 500 μM Cd concentration condition, the colonization of AMF in roots decreased, and the alleviating effect of AMF was not significant. Ultrastructural observations showed that Cd is abundant in regular lumps and strips in the cross-section of E. grandis root cell. AMF protected plant cells by retaining Cd in the fungal structure. Our results suggested that AMF alleviated Cd toxicity by regulating plant physiology and altering the distribution of Cd in different cell sites.


Introduction
Cadmium (Cd) accumulation in soil has become a serious global concern with pronounced harmful effects on water, agricultural productivity, and human health [1]. In dealing with Cd pollution, people developed phytoremediation technology, which uses metal-accumulating plants to remove toxic metals from contaminated soil [2,3]. However, hyperaccumulator plants are mostly herbaceous [4]. Herbaceous' vulnerability to soil moisture, salinity, and pH greatly limited its practical application [5]. It is crucial to find a woody plant with high biomass, rapid growth, and good economic returns that can be used for the phytoremediation of heavy-metal-contaminated soil [6]. Eucalyptus grandis (E. grandis) is one of the most widely distributed fast-growing timber forests with a long taproot, a strongly developed root system, and large biomass [7]. Some researchers reported that arbuscular mycorrhizal fungi (AMF) symbiosis with E. grandis can enhance the heavy metal resistance of plants [8,9]. Therefore, E. grandis contains great potential and ecological value as a bio-remediation tree for heavy-metal-contaminated soil [10]. However, the extent of Cd tolerance in E. grandis and how Cd is transported at the subcellular level remain to be investigated.
AMF can form a symbiotic relationship with 85% of plant roots, improves the resistance of host plants towards heavy metal toxicity, and enhances plant stability under

Experiment Design
Pot experiments were undertaken at the State Key Laboratory of Conservation and Utilization of Subtropical Agro-Bioresources (Guangzhou, China). A mixture of 0.6 mm sand and vermiculite was sterilized at 121 • C for 2 h to serve as the culture medium. The range of tolerance of E. grandis was obtained through preliminary experiments and previous data from our research group. Therefore, our experiment included five levels of Cd concentration: 0, 50, 150, 300, and 500 µM; two inoculation treatments: non-mycorrhizal treatment (NM) and AMF inoculation (AM). Each treatment was replicated six times, resulting in a total of 60 rectangular pots. The inoculation containing 400 AMF spores was added to the substrate of the AM group, and the same amount of spore-free filtrate was applied to the control group. After AMF inoculation, all seedlings were normally watered 30 mL each day, and LA nutrient solution with low phosphorus content (contains one-tenth of phosphorus) was poured once each 3 days, 50 mL per pot. After 45 days, confirmed the colonization, then started heavy metal treatment. Different concentration of cadmium chloride (CdCl 2 ) was applied once every 5 days, 50 mL each time, for a total of 8 times. After 40 days of heavy metal stress, the samples were collected for the determination of relevant indicators.

Growth Indicators Determination 2.3.1. Biomass
Five seedlings were randomly selected for each treatment, and the surfaces of roots, stems, and leaves were gently washed with tap water to drain the surface moisture. The fresh weight of the root and shoot of E. grandis was measured by electronic balance (accurate to 0.001 g). Part of the weighed plant samples was placed at 105 • C for 10 min, then continuously placed at 70 • C for 72 h until constant weight and measured the dry weight of the shoot and root parts of the plant.

Mycorrhizal Colonization
The improved trypan blue staining method was used for staining using the method [23]. The grid-line crossing method [24] was used to measure the colonization of AMF in roots, and related indexes such as total colonization rate of roots, arbuscular colonization rate, and vesicle colonization rate were recorded.

Chlorophyll Fluorescence Parameters
In total, 5 plants were randomly selected from each treatment, and dark adaptation was conducted for 30 min. The 5th-6th leaves from top to bottom were selected and determined by a dual-channel chlorophyll fluorescence analyzer (Dual-PAM-100, WALZ, Bavaria, Germany). These chlorophyll fluorescence parameters were adopted from the following equations defined by Rascher et al. [25].
where F m and F 0 are the maximal and minimal fluorescence values of dark-adapted leaves after 30 min, respectively, F v is the variable fluorescence, Fm is the maximal fluorescence of the light-adapted leaves. ETR is the electron transport rate, and qP is the photochemical quenching coefficient; these two indicators are directly measured by the instrument.

Cd Concentration Analysis
Parts of the roots and leaves were washed with 10 mmol L −1 EDTA (pH 8.0) and rinsed with ddH 2 O 2 to remove the metal ions from the root surface [26], oven-dried at 105 • C for 30 min, followed by 70 • C until constant masses, weighed and ground with a stainless-steel mill, then passed through a 0.1 mm nylon sieve. About 0.1 g of the plant sample was digested using the HNO 3 -HClO 4 (3:1) method [27]. The digested solutions were washed with ddH 2 O 2 in a 15 mL centrifuge tube. Cd quantification was performed with an Inductively Coupled Plasma Emission Spectrometer (prodigy 7, Leeman, Hudson, NH, USA). The following formulae were used to calculate the key parameter that was analyzed [28]. Translocation factor (TF) = Cd shoots /Cd roots . Cd shoots denotes the Cd concentration in shoots, while Cd roots denotes the Cd concentration in roots.

Cd Localization in Roots of E. grandis
Ultrathin section from the NM and AM-treated E. grandis root cell was negatively stained with 2% uranyl acetate and 1% lead citrate. The cross-section of AMF-E. grandis symbiont cell and the distribution of Cd in E. grandis roots were examined under a Field Emission Transmission Electron Microscope (Talos F200S, FEI company, Hillsboro, OR, USA).

Statistical Analysis
SPSS 22.0 statistical program (SPSS Inc., Chicago, IL, USA) was used to statistically analyze the growth parameters, chlorophyll fluorescence parameters, AMF colonization, and Cd concentration in NM/AM. All data met the normality and homogeneity of variance assumptions and were analyzed by ANOVA with means comparisons according to Duncan's multiple range test (p < 0.05). For the biomass, chlorophyll fluorescence parameters, and Cd concentration of plants, two-way ANOVAs were used to assess the effects of "AMF" and "Cd treatment". Graphs were prepared using SigmaPlot version 12.3 (Systat Software Inc., San Jose, CA, USA).

Effects of Different Cd Concentrations on AMF Colonization
Different Cd concentrations affected the AMF colonization on E. grandis roots. The proportion of arbuscule was relatively high under non-stress conditions. The proportion of vesicles and hyphae increased with the increase in Cd concentration. Under 500 µM Cd concentration condition, a large amount of degraded arbuscule was observed ( Figure S3). Compared with the non-stress group, the total colonization rate increased significantly when Cd concentration was 50, 150, and 300 µM, which reached 67.40%, 68.67%, and 66.66%, respectively. However, when the Cd concentration reached 500 µM, the total colonization rate decreased to 63.80% ( Figure 1A). The colonization rate of arbuscule decreased with the increase in Cd concentration. Compared with the non-stress group, the colonization rate of arbuscule decreased by 14.40%, 39.70%, 53.00%, and 52.68% under 50, 150, 300, and 500 µM Cd concentration conditions ( Figure 1B). The colonization rate of vesicles increased significantly with the increase in Cd concentration and reached the maximum value at 500 µM, which was 156.28% higher than that under non-stress conditions ( Figure 1C).

Effects of AMF on E. grandis Growth Parameters under Different Cd Concentrations
We found that under Cd stress, E. grandis could grow under all concentration conditions without AMF colonization, but plants showed stunting, such as wilting and red leaves. In the high Cd concentration treatment (500 μM) group, the leaves of the plant even showed a lot of litter ( Figure S4). The AM group exposed to Cd stress also showed

Effects of AMF on E. grandis Growth Parameters under Different Cd Concentrations
We found that under Cd stress, E. grandis could grow under all concentration conditions without AMF colonization, but plants showed stunting, such as wilting and red leaves. In the high Cd concentration treatment (500 µM) group, the leaves of the plant even showed a lot of litter ( Figure S4). The AM group exposed to Cd stress also showed Cd toxicity, such as decreased height and red leaves, but the toxicity degree was significantly less than the NM group ( Figure S5).
After 40 days of Cd treatment, the dry weight of both shoots and root of E. grandis decreased significantly with the increase in Cd concentration, and AMF could significantly alleviate the reduction of biomass. The mycorrhizal efficiency was most significant under 300 µM Cd concentration condition. The dry weight of shoots and roots in the NM group decreased by 47.84% and 49.59% compared with the non-stress group. However, the dry weight of shoots in AM group only reduced by 34.97% and 36.51% compared with the non-stress condition ( Figure 2). When the concentration of Cd increased to 500 µM, there was no significant difference in dry weight between the NM and AM groups, and the mycorrhizal efficiency of AMF was insignificant. The effects of AMF, Cd reached significant levels (p < 0.05) on all tested biomass of root and shoot, but their interactions showed no significant effect on those parameters. Root colonization (A), arbuscules colonization (B), and vesicle colonization (C) of E. grandis inoculated with R. irregularis grown under different Cd concentrations (mean ± SE, n = 4). By ANOVA, both root colonization (A), arbuscules colonization (B), and vesicle colonization (C) were significantly (p < 0.05) affected by Cd concentration. The same lowercase letters above the columns indicate no significant (p < 0.05) differences among all treatments by Duncan's multiple range test.

Effects of AMF on E. grandis Growth Parameters under Different Cd Concentrations
We found that under Cd stress, E. grandis could grow under all concentration conditions without AMF colonization, but plants showed stunting, such as wilting and red leaves. In the high Cd concentration treatment (500 μM) group, the leaves of the plant even showed a lot of litter ( Figure S4). The AM group exposed to Cd stress also showed Cd toxicity, such as decreased height and red leaves, but the toxicity degree was significantly less than the NM group ( Figure S5).
After 40 days of Cd treatment, the dry weight of both shoots and root of E. grandis decreased significantly with the increase in Cd concentration, and AMF could significantly alleviate the reduction of biomass. The mycorrhizal efficiency was most significant under 300 μM Cd concentration condition. The dry weight of shoots and roots in the NM group decreased by 47.84% and 49.59% compared with the non-stress group. However, the dry weight of shoots in AM group only reduced by 34.97% and 36.51% compared with the non-stress condition ( Figure 2). When the concentration of Cd increased to 500 μM, there was no significant difference in dry weight between the NM and AM groups, and the mycorrhizal efficiency of AMF was insignificant. The effects of AMF, Cd reached significant levels (p < 0.05) on all tested biomass of root and shoot, but their interactions showed no significant effect on those parameters.  . AM and NM, respectively, represent inoculation with AMF and non-inoculation control. The same lowercase letters above the columns indicate no significant (p < 0.05) differences among all treatments by Duncan's multiple range test. Significant effect of two-way ANOVA: *** p < 0.001; ns: no significant effect.

Effects of AMF on E. grandis Photosynthesis Parameters under Different Cd Concentrations
Under Cd stress, AMF could significantly increase ΦPSII, Fv /Fm , ETR, and qP ( Figure 3). AMF inoculation significantly increased the PSII under non-stress and low Cd stress (50 and 150 µM); compared with the NM group, AM group increased by 43.33%, 50.69%, and 65.09%, respectively ( Figure 3A). Fv /Fm decreased with the increase in Cd concentration; it decreased by 26.88% and 31.36% Cd concentration of 300 µM and 500 µM compared with that under non-stress condition, and AMF inoculation significantly increased Fv /Fm by 37.01% and 43.71% ( Figure 3B). Meanwhile, AMF inoculation significantly increased the ETR under non-stress and low Cd stress (50, 150 µM), compared with the NM group, AM group increased by 43.19%, 52.07%, and 64.67%, respectively ( Figure 3C). The qP was significantly increased by AMF inoculation under non-stress and low concentration Cd stress (50 and 150 µM); AMF inoculation significantly increased the qP, compared with the NM group, AM group increased by 39.49%, 23.95%, and 55.58% ( Figure 3D). The effects of AMF and Cd reached significant levels (p < 0.05) on all tested chlorophyll fluorescence parameters, but their interactions showed no significant effect on those parameters. creased Fv′/Fm′ by 37.01% and 43.71% ( Figure 3B). Meanwhile, AMF inoculation significantly increased the ETR under non-stress and low Cd stress (50, 150 μM), compared with the NM group, AM group increased by 43.19%, 52.07%, and 64.67%, respectively ( Figure  3C). The qP was significantly increased by AMF inoculation under non-stress and low concentration Cd stress (50 and 150 μM); AMF inoculation significantly increased the qP, compared with the NM group, AM group increased by 39.49%, 23.95%, and 55.58% (Figure 3D). The effects of AMF and Cd reached significant levels (p < 0.05) on all tested chlorophyll fluorescence parameters, but their interactions showed no significant effect on those parameters.  . AM and NM, respectively, represent inoculation with AMF and non-inoculation control. The same lowercase letters above the columns indicate no significant (p < 0.05) differences among all treatments by Duncan's multiple range test. Significant effect of two-way ANOVA: *** p < 0.001; ** p < 0.01; ns: no significant effect.

Effects of AMF on the Cd Absorption of E. grandis
There were differences in total Cd concentration in E. grandis and Cd concentration in shoot and root under different Cd concentration conditions (Figure 4). The Cd concentration in the plantlet increased significantly with the increase in Cd concentration, and the effect of Cd reached significant levels (p < 0.05) on tested total Cd concentration in E. grandis, but the effect of AMF their interactions showed no significant effect on those parameters ( Figure 4A). However, AMF inoculation significantly increased Cd concentration in the root while significantly reducing Cd concentration in shoot; the effects of AMF and Cd reached significant levels (p < 0.05) on tested Cd concentration in both shoot and root ( Figure 4B,C). Under 300 µM Cd concentration condition, the effect of AMF inoculation was the most significant, and the concentration of Cd in the shoot was reduced by 64.08% ( Figure 4B). AMF reduced the translocation factor of Cd. After being treated with 50, 150, 300, and 500 µM, the translocation factor in AM group decreased by 56.41%, 62.89%, 66.67%, and 42.79%, respectively ( Figure 4D). and Cd reached significant levels (p < 0.05) on tested Cd concentration in both shoot and root ( Figure 4B, C). Under 300 μM Cd concentration condition, the effect of AMF inoculation was the most significant, and the concentration of Cd in the shoot was reduced by 64.08% ( Figure 4B). AMF reduced the translocation factor of Cd. After being treated with 50, 150, 300, and 500 μM, the translocation factor in AM group decreased by 56.41%, 62.89%, 66.67%, and 42.79%, respectively. ( Figure 4D). irregularis under different Cd concentration (mean ± SE, n = 4). AM and NM, respectively, represent inoculation with AMF and noninoculation control. The same lowercase letters above the columns indicate no significant (p < 0.05) differences among all treatments by Duncan's multiple range test. Significant effect of two-way ANOVA: *** p < 0.001; ** p < 0.01; ns: no significant effect.

Effects of AMF and Cd Stress on E. grandis Root Cell Ultrastructure
We found that under 500 μM Cd concentration condition, the morphology of NM root cortex cells changed, most of the cells showed irregular strip shape, some cells burst . AM and NM, respectively, represent inoculation with AMF and non-inoculation control. The same lowercase letters above the columns indicate no significant (p < 0.05) differences among all treatments by Duncan's multiple range test. Significant effect of two-way ANOVA: *** p < 0.001; ** p < 0.01; ns: no significant effect.

Effects of AMF and Cd Stress on E. grandis Root Cell Ultrastructure
We found that under 500 µM Cd concentration condition, the morphology of NM root cortex cells changed, most of the cells showed irregular strip shape, some cells burst (c in Figure 5) or even collapsed (b in Figure 5), and a large number of gray black and dark black cells (a in Figure 5) appeared compared with the non-stress group, and that the dark black lipids were concentrated in the lateral cells of the stele and the lateral cells of the endodermis of the E. grandis roots. We suspected this deposition site was Cd. Compared with the NM group, it can be seen that gray black cells in AM group decreased obviously, and we found the arbuscular structure of AMF entered the cells of the E. grandis root system and were able to occupy the whole cell (d in Figure 5), which was relatively intact compared to other cells that are deformed, ruptured or even collapsed. Hypha of AMF could also be observed under field emission transmission electron microscopy.
At the subcellular level in E. grandis root without AMF colonization, the cell structure was obviously incomplete, cell membrane breakage resulting in cell wall collapsed and tissue breakage ( Figure 5C). Cd toxicity has a great effect on NM cell structure. We found AMF inoculated in E. grandis root, and the symbiont cell was complete and regular compared with Cd-poisoned cells; AMF could effectively alleviate cell deformation and collapse caused by Cd toxicity ( Figure 5D). In the local figure of fungal structures in E. grandis roots, it can be seen that 5D was arbuscular cell, and 5E and 5H were hypha structures. Hexagonal crystals with regular shape were deposited around the arbuscular cells (g in Figure 5), which we suspected to be complex precipitation; the sites indicated by arrows h and j were suspected of Cd deposition in hypha. black lipids were concentrated in the lateral cells of the stele and the lateral cells of the endodermis of the E. grandis roots. We suspected this deposition site was Cd. Compared with the NM group, it can be seen that gray black cells in AM group decreased obviously, and we found the arbuscular structure of AMF entered the cells of the E. grandis root system and were able to occupy the whole cell (d in Figure 5), which was relatively intact compared to other cells that are deformed, ruptured or even collapsed. Hypha of AMF could also be observed under field emission transmission electron microscopy. At the subcellular level in E. grandis root without AMF colonization, the cell structure was obviously incomplete, cell membrane breakage resulting in cell wall collapsed and tissue breakage ( Figure 5C). Cd toxicity has a great effect on NM cell structure. We found AMF inoculated in E. grandis root, and the symbiont cell was complete and regular We performed energy spectrum analysis on the parts of NM E. grandis cells, which were suspected to be Cd deposition ( Figure 6A) and collapsed cells ( Figure 6E). The results are shown in Figure 6D,H; the occurrence of a Cd peak indicates that there are indeed a large number of Cd deposits in these two sites, and the distribution range of Cd is shown in Figure 6C,G. We can clearly see that Cd is uniformly concentrated in the gray and black parts and the collapsed cell wall under TEM-EDS; the results showed that the broken and collapsed cells in NM roots were indeed caused by the toxic effect of Cd, and we can preliminarily speculate that the deposition position of Cd in the root cells without AMF inoculation is in the dark black cells in the section. However, the EDS result of AM root showed that Cd was abundant in vesicle cells and existed as regular strips ( Figure 6K); the degree of cell collapse was obviously less than the NM group ( Figure 6I). With AMF colonization, Cd-poisoned cells maintained relatively intact cell morphology and structure. These results suggest that AMF could help E. grandis root cells retain Cd, thus reducing the toxicity of Cd to E. grandis cells.
liminarily speculate that the deposition position of Cd in the root cells without AMF inoculation is in the dark black cells in the section. However, the EDS result of AM root showed that Cd was abundant in vesicle cells and existed as regular strips ( Figure 6K); the degree of cell collapse was obviously less than the NM group ( Figure 6I). With AMF colonization, Cd-poisoned cells maintained relatively intact cell morphology and structure. These results suggest that AMF could help E. grandis root cells retain Cd, thus reducing the toxicity of Cd to E. grandis cells.  In addition, we found the distribution and form of Cd in cross sections of E. grandis root by analyzing the areas of Cd enrichment sites in cells treated with Cd at 500 µM under field emission transmission electron microscopy. The bright patches are the locations of Cd in the energy spectrum. The results of the EDS analysis showed that peaks of C, O, Os, Cu, and Cd appeared ( Figure 7C,F). The samples' biological nature resulted in the appearance of C and O peaks in the figure. The carrier network of transmission electron microscope uses the Cu network, so the Cu peak appears. Because the sample was stained with osmium, the Os peak appeared. The appearance of Cd peaks proves that these bright patches are indeed made of Cd, and Figure 7B,E show the form of Cd; Cd are abundant in regular lumps and strips.
Cd in the energy spectrum. The results of the EDS analysis showed that peaks of C, O, Os, Cu, and Cd appeared ( Figure 7C,F). The samples' biological nature resulted in the appearance of C and O peaks in the figure. The carrier network of transmission electron microscope uses the Cu network, so the Cu peak appears. Because the sample was stained with osmium, the Os peak appeared. The appearance of Cd peaks proves that these bright patches are indeed made of Cd, and Figure 7B,E show the form of Cd; Cd are abundant in regular lumps and strips.

AMF Improved the Growth and Photosynthetic Efficiency of E. grandis under Cd Stress
In the present study, we found that the biomass of E. grandis decreased with the increase in Cd concentration, Cd toxicity inhibited plant growth, and AMF colonization strongly enhanced the biomass of E. grandis under Cd stress except for 500μM. AMF are widely believed to support plant establishment in soils contaminated with heavy metals because AM symbiosis with plants promotes the growth of the host [29,30]. In this study, R. irregularis inoculation enhanced plant development under Cd stress, which was manifested by higher shoot and root biomass.
Chlorophyll fluorescence parameters are important indicators to show plants' responses and adaptations toward heavy stress [31]. Our results indicated that E. grandis showed significantly lower Fv′/Fm′ and qP under Cd stress, which infers the negative impact of Cd on photosynthesis. Moreover, the leaves of E. grandis inoculated with R. irregularis maintained higher ΦPSII, ETR, and qP values under Cd stress. A previous study showed that the loss of photosynthesis performance ΦPSII was caused by the decrease in Fv′/Fm′ and qP, which indicates a reduced consumption of NADPH and ATP in the Calvin cycle due to reduced demand of sugars in other plant parts caused by Cd or inhibition of

AMF Improved the Growth and Photosynthetic Efficiency of E. grandis under Cd Stress
In the present study, we found that the biomass of E. grandis decreased with the increase in Cd concentration, Cd toxicity inhibited plant growth, and AMF colonization strongly enhanced the biomass of E. grandis under Cd stress except for 500 µM. AMF are widely believed to support plant establishment in soils contaminated with heavy metals because AM symbiosis with plants promotes the growth of the host [29,30]. In this study, R. irregularis inoculation enhanced plant development under Cd stress, which was manifested by higher shoot and root biomass.
Chlorophyll fluorescence parameters are important indicators to show plants' responses and adaptations toward heavy stress [31]. Our results indicated that E. grandis showed significantly lower F v /F m and qP under Cd stress, which infers the negative impact of Cd on photosynthesis. Moreover, the leaves of E. grandis inoculated with R. irregularis maintained higher ΦPSII, ETR, and qP values under Cd stress. A previous study showed that the loss of photosynthesis performance ΦPSII was caused by the decrease in F v /F m and qP, which indicates a reduced consumption of NADPH and ATP in the Calvin cycle due to reduced demand of sugars in other plant parts caused by Cd or inhibition of enzymes of the Calvin cycle [11]. Reduction in the quantum yield of photosystem II and electron transport rate and the increase in the non-photochemical quenching and steady-state chlorophyll fluorescence showed that the capture of light energy by plants was missed out in the form of the non-fluorescence quenching [9]. In this research, F v /F m , ΦPSII, ETR, and qP in E. grandis increased after R. irregularis inoculation compared with non-mycorrhizal E. grandis under cd stress, suggesting that AMF colonization alleviated the cd stress in E. grandis while significantly increasing photosynthetic protection.
High concentrations of metals can inhibit AMF spore germination and extra-root mycelial growth, thus affecting the colonization of AMF in plant roots [32]. However, some researchers have reported different results. For example, the colonization rates of Rhizophagus intraradices to wild tobacco were increased from 14 to 81% when soil Zn levels were increased from 0 to 250 mg kg −1 [33]. Due to the capacity of the AMF isolate to inhabit contaminated soils as well as mycorrhizal dependency, the mycorrhizal colonization observed can be partly explained [21]. AMF has a certain tolerance to heavy metal stress, and a high concentration of Cd stress has a certain impact on the growth and development of AMF. Thus, high concentrations of heavy metals decrease the colonization of AMF in plant roots, but such findings may differ due to a wide variety of reasons, such as the compatibility of AMF species and plants, element concentration of metal and oxidation state, and environmental conditions [34,35]. Our results indicated that Cd treatment (50, 150, 300 µM) significantly increased AMF colonization compared with non-Cd treatment. The reason for this may be the vesicles and hyphae of AMF are used for chelating heavy metals after the addition of Cd. While under a Cd concentration of 500 µM, high concentrations of Cd limited the growth of AMF, root colonization decreased, and AMF had no significant effect on growth parameters and photosynthetic efficiency.

AMF Mobilizes the Distribution and Transportation of Cd in E. grandis
The mycorrhizal efficiency resulted in a biomass allocation mechanism with a preference for the root system, ensuring tolerance, enrichment, and immobilization of the root system to toxic trace element contamination [36,37]. AMF was demonstrated to affect heavy metals bioavailability in the host plants and promote HMs retention in the roots, improving shoot biomass by restricting translocation to the aerial parts [21,38]. We observed that although there was no significant difference in the total Cd content between mycorrhizal and non-mycorrhizal plants, the Cd concentration in the roots of mycorrhizal plants was significantly higher than that in the shoots, indicating that AMF colonization significantly inhibited the migration of Cd from the roots to the shoots, thus limiting the accumulation of Cd in the photosynthetic tissues and effectively alleviating the toxic effect of Cd on the shoots.
On the other hand, AMF colonization has different effects on the distribution and transportation of heavy metals in plants [39,40]. Qiao et al. [41] showed that after being inoculated with Funneliformis mosseae, Medicago sativa L. had higher Co and Pb concentrations, and AMF inoculation promoted HMs translation to shoot. Citterio et al. [42] reported the influence of Funneliformis mosseae inoculation on the Cd, Ni, and Cr uptake of Cannabis sativa L. under heavy metal and found that the concentration of heavy metal was not affected by inoculating F. mosseae. Cui et al. [43] found R. irregularis effectively impacted the partitioning of Mg, Cu, and Zn accumulation and partition, including increased Mg and decreased Cu and Zn relative concentrations in shoots of soybean. Hence, the effects of AMF inoculation on the distribution and transportation of heavy metal are associated with AMF and plant species [20]. In our study, R. irregularis played an important role in regulating the distribution and transport of Cd in E. grandis, protecting the photosynthetic system by accumulating more Cd in the root and reducing Cd transport to the shoot. Therefore, E. grandis symbiosis with R. irregularis is a feasible strategy for the remediation of Cd-contaminated soils.

Damage of Cell Ultrastructure in E. grandis Root by Cd and Positive Effect of AMF Colonization
Plants' detoxification to heavy metal by fixing heavy metal particles in cell structures (vacuoles, cell walls), which are not involved in important physiological and biochemical processes [44]. Here, we investigated the altered ultrastructure of E. grandis cells and hypothesized that AMF jointly alleviate Cd toxicity by altering the distribution of Cd in different cell sites. We found that Cd are abundant in regular lumps and strips in the cross-section of E. grandis root cell; Cd was present in some intact vacuoles and in the walls of some collapsed cells. This result is similar to the findings of Kiran et al. [45], who found that Cd in the root system of Brassica rapa subsp. chinensis L. mostly exists in the vacuole or attached to the cell wall and exhibited exudates of Cd-dense material. Cd was observed in the roots of mycorrhizal plants in the form of aggregated regular strips and blocks attached to the cell walls or in vacuoles, which reduced the toxicity of Cd to the plant cells. Meanwhile, we found Cd possibly induced alterations in the ultrastructure of endodermal and stele cells. In the entire cortex of E. grandis, especially in cells located closer to the stele, there appeared a large number of cells containing dark black material (stained with uranium dioxy acetate and lead citrate), and these cells showed deformation or even rupture, and they showed electron-dense cytoplasm, which was preliminarily speculated as the deposition location of Cd, and we speculated that the black deposits were lipids and that the dark black lipids were concentrated in the lateral cells of the stele and the lateral cells of the endodermis of the E. grandis roots. These results agree with the study of Katarzyna Głowacka et al. [46]; they noticed in almost all tissues of the root was an increased number of oil bodies, while the oil bodies were mainly observed in the cytosol of the vascular parenchyma cells, the cytoplasm of other stele cells, and in the cortical cells treated with Cd. It should be noted that high concentrations of Cd in the root epidermis have been reported in previous studies [33,47]. A large amount of Cd might accumulate between the epidermis and outermost layer of the cortex, and a higher concentration of Cd within the stele implies that a considerable fraction of the Cd absorbed by the root has entered the vascular bundle in the root [45]. In addition, our observations were similar to Katarzyna Głowacka et al. [46], the roots exposed to Cd, a strong H 2 O 2 -DAB dependent reaction was also seen in the entire cortex, especially in cells located closer to the stele. Thus, Cd ions tend to accumulate in the cells located closer to the stele in the cross-section of the E. grandis root cell and exist in regular lumps and strip cells, which we suspected to be lipid-containing structures. The lightening of the color of this part of the cells under TEM after inoculation with AMF also indicates that AMF symbiosis reduced Cd transport through the mid-column to the above-ground part.
A previous study reported that AMF improves heavy metal tolerance in plants due to its ability to sequester heavy metal ions in their intraradical mycelia [20]. It has also been shown that this toxic metal was mainly retained in the fungal structure, particularly in the arbuscules, and did not appear to be delivered to plant cells [22]. Our results indicated that cells containing lipids material significantly decreased in the root inoculated with R. irregularis, and we found that the deposits of Cd were mainly concentrated around the arbuscular structure, in the form of a regular lens, or in the hypha structure. Thus, at the subcellular level, E. grandis symbiosis with R. irregularis could protect the root cell structure of the plant by concentrating Cd around the arbuscular structure or in the hypha structure and effectively maintaining the integrity of the nearby cell morphology. This may be an effective strategy for R. irregularis to enhance the heavy metals tolerance of E. grandis.

Conclusions
Our study indicated that AMF could significantly alleviate Cd toxicity by enhancing the biomass, improving photosynthetic efficiency, and reducing the transfer of Cd to the shoot. However, when Cd concentration rises to 500 µM, the mycorrhizal efficiency is limited, the root colonization decreased, and the proportion of arbuscule decreased significantly, thus reducing the effect of alleviating Cd toxicity in E. grandis. From the cellular ultrastructure perspective, AMF retained Cd in the symbiotic cell so as to reduce the Cd toxicity to the root cell of E. grandis. This may be the mechanism by which AMF helps E. grandis resist heavy metal toxicity at the subcellular level. Our work helps to explain the mechanism of Cd toxicity alleviation by R. irregularis and provides a theoretical reference for using woody in heavy-metal-polluted soil remediation. Interestingly, hexagonal crystals with regular shapes were observed in our research. In the future, its composition and whether it is involved in AMF chelating heavy metals should be given more attention.