In southern Chile, acidic volcanic soils (Andisols and Ultisols) are the predominant soil types supporting the bulk of agricultural and forestry production. Andisols include modern and recent ash deposits, and Ultisols correspond to ancient deposits (Andrade et al., 2011). Soil samples were collected from extensive wheat cropping areas managed by Mapuche communities in 16 locations from La Araucania (Figure 1A; Table 1). Nine samples (number 3, 4, 5, 7, 10, 12, 13, 14, 15, and 16) were taken from soils with a long rotation history between wheat monoculture and natural pasture for more than 10 years, and six samples (number 2, 6, 8, 9, 11, and 12) were taken from soils with wheat monoculture including oat rotation. An additional sample number 1 was taken from a Ggt-conducive soil with wheat, including clover rotation, and used as positive control. Parent material from soils 1 to 10 was classified as Andisol, whereas 11–16 were classified as Ultisols.

Samples were collected from rhizosphere and bulk soil at 0–20 cm depth, and then stored in a cold room at 5°C until usage. Soil sample chemical properties were determined as follow. Briefly, available P (P_Olsen) was extracted by using 0.5 M Na-bicarbonate and analyzed by using the molybdate method (Murphy and Riley, 1962). Organic matter contents were estimated by wet digestion (Walkley and Black, 1934). Soil pH was measured in 1:2.5 soil/deionized water suspensions. Exchangeable potassium (K⁺), calcium (Ca²⁺), magnesium (Mg²⁺), and sodium (Na⁺) were extracted with 1 M ammonium acetate (CH₃COONH₄) at pH 7.0 and analyzed by flame atomic adsorption spectrophotometry (FAAS) (Warncke and Brown, 1998). Exchangeable aluminum (Al³⁺) was extracted with 1 M KCl and analyzed by FAAS (Bertsch and Bloom, 1996). All samples analyses were made in triplicate. To group and determine significant differences between samples based on their chemical properties, data were imported into the PRIMER 7 software (PRIMER-E Ltd, Ivybridge, UK), transformed and normalized using square-root followed by a log (Xþ1) transformations (Lee et al., 2012). Then, a distance matrix was generated based on Euclidean distances and samples were grouped by hierarchical clustering (group average), and then visualized by principal component analysis (PCA).

Bacterial community compositions in rhizosphere and bulk soil samples were examined by denaturing gradient gel electrophoresis (DGGE), according to Iwamoto et al. (2000). Total genomic DNA was extracted from 0.5 to 1 g of soil samples using the PowerSoil® DNA Isolation Kit (Mo-Bio Laboratories, Carlsbad, CA, USA), according to manufacturer's instructions. The 16S rRNA gene fragments were amplified by touchdown PCR, using EUBf933-GC/EUBr1387 primer set (Iwamoto et al., 2000). DGGE analysis was performed using a DCode system (Bio-Rad Laboratories, Inc., USA). The PCR product (20 μL) was loaded onto a 6% (v/v) polyacrylamide gel with a 40–70% gradient (urea and formamide). Electrophoresis was run for 12 h at 100 V. Banding profiles were visualized by staining the gel 1:10.000 (v/v) with SYBR Gold (Molecular Probes, Invitrogen Co., USA) for 30 min, followed by image capture using GelDoc-It^TS2 Imager (UVP, Upland, CA, USA). DGGE banding profile clustering, using a dendrogram, was also carried out by using Phoretix 1D analysis software (TotalLab Ltd., UK). The correlation between bacterial communities (biological parameters) and chemical soil properties (ecological parameters) was visualized by non-metric multidimensional scaling (MDS) analysis using Primer 7 + Permanova software (Primer-E Ltd., Ivybridge, UK) (Clarke, 1993). The in silico analysis was also used to estimate the bacterial diversity by richness (S), Shannon–Wiener, and dominance by Simpson Index (D), represented by 1-D or 1-λ (Sagar and Sharma, 2012).

Ggt occurrence in soil samples: DNA extracts from soil samples were subjected to PCR using the primer set NS5 (5′-AAC TTA AAG GAA TTG ACG GAA G-3′) and GGT-RP (5′-TGC AAT GGC TTC GTG AA-3′) designed by Fouly and Wilkinson (2000) specifically for Ggt. The PCR conditions were as follow: an initial denaturation at 93°C for 3 min, followed for 93°C for 1 min, 52°C for 1 min, and 72°C for 1 min to 35 cycles, and finally with 72°C for 5 min. All soil samples were tested in triplicate, and pure G. graminis var tritici (Andrade et al., 2011) and Aspergillus niger DNA (code CCT-UFRO 15.62), obtained from La Frontera University Type Strain Culture Collection (http://ccct.ufro.cl/), were used as positive and negative controls, respectively. The presence of Ggt in soil samples showing positive Ggt reaction was also confirmed by the presence of take-all disease symptoms, chlorosis, and blackening roots in wheat seedlings in the pot assays.

Putative Ggt-suppressive soil screening was performed by two in vitro inhibition tests using rhizosphere soil samples as follows:

Data normality was analyzed according to Kolmogorov's test. Data obtained in Section In vitro Inhibition Test on Solid Media (in vitro plate assay) were analyzed by a one-way analysis of variance (ANOVA) and compared by Tukey test, using SPSS software (SPSS, Inc.). Comparisons between inoculated and non-inoculated samples from screening 2 were made, and Student t-test was used for related samples with 95% confidence interval. For the greenhouse assay multivariate analysis of variance (MANOVA) and comparisons were carried out for each set with Tukey's test by SPSS software (SPSS, Inc.). Values were given as means ± standard errors. Differences were considered significant when the P value was lower than or equal to 0.01. The microbial diversity analysis was described above.

In order to determine the chemical composition of the collected soils, chemical analyses were performed using triplicate samples of each soil. The main chemical parameters that were measured are shown in Table 2. In general, soil samples showed values of available P from 5.6 (soil 13) to 60 mg kg⁻¹ (Soils 1 and 4). The pH ranged from 5.0 (soils 11 and 12) to 6.4 (soil 15). The OM contents varied from 6% (soil 14) to 15% (soils 6, 7, and 15). The higher values of S bases and Al saturation were observed in soil 15 (29.4 cmol₍₊₎ kg⁻¹) and soil 11 (14%), respectively; whereas lower values were observed in soil 6 (4.7 cmol₍₊₎kg⁻¹) and soil 15 (0 cmol₍₊₎kg⁻¹). In addition, the PCA analysis showed that soils were grouped based on their chemical composition and soil classification, Andisol and Ultisol (Figure 1B). Several soil groups were formed, soils collected from Perquenco, Las Cardas, Momberg, Quilaco, Membrillar, and Lufquentue clustered together (soils 1, 2, 3, 4, 5, 7, 9, 10, and 16, respectively), soils from Quilaco (6) and Boyeco (11 and 12), and three soils collected from Lufquentue (soils 13, 14, and 15) and Quilaco (soil 8) did not cluster with any other group.

Rhizosphere community composition is highly related to soil classification as revealed by MDS, in which microbiology and soil chemical/environmental properties were analyzed (Figure 2A). Samples from Andisol and Ultisol were notably different from each other, with 55% similarity. According to the Spearman correlation, Ultisol soils were more significantly related with chemical parameters than Andisol soils (r² = 0.90 and r² = 0.59, respectively, Table 3). Bulk soils were also separated according to the chemical soil composition, but this difference was not significant, and all samples were grouped at 55% (Figure 2B). In this sense, both Andisol and Ultisol were equally related with soil chemical parameters (r² = 0.83, Table 3).

Differences in bacterial community structures between bulk and rhizosphere soil were revealed by MDS analysis, based on DGGE banding profiles. In relation to bulk soils, the nMDS analysis revealed the existence of major groups at 40% similarity formed by rhizosphere soils indistinctly grouped, all correlated among them. In general, bulk soils were separated into two main groups formed mainly by Andisol (soil 1, 2, 3, 4, 5, 6, 7) and Ultisol soils (11, 12, 13, 14, 15, 16) (Figure 3).

Regarding the microbial diversity in bulk and rhizosphere soils (Supplementary Figure 2), in general, the Shannon index (H') showed values <2.0 for bulk (except soils 5 and 6 from Quilaco) whereas it reached values ~2.5 for rhizosphere soil, indicating a lower diversity in bulk than in rhizosphere soils. A similar trend was observed in the case of species number (S). The lowest diversities (<1.0) and species richness (S) were observed in bulk soils from Membrillar (soils 9 and 10) whereas highest diversity values were obtained in rhizosphere soils from Quilaco (soil 5 and 6). As for bulk soils, rhizosphere soils taken from Membrillar also showed lower diversity values (≤2.0). In contrast, less dominance values in rhizosphere soils compared with bulk soils were also observed by Simpsons (D) index represented by 1-D, in which the lower values indicate major dominance of species. Thus, samples 9 and 10, which showed less diversity according to the Shannon index, also showed major dominance of species. Therefore, bulk soils showed lower biodiversity and major dominance compared to rhizosphere soils (Supplementary Figure 2), and we observed a direct Pearson correlation between both indexes (P < 0.01, data not shown).

According to the in vitro inhibition test on solid media (Figure 4A and Supplementary Figure 1A), four soils from Las Cardas (soils 2 and 3), Boyeco (soil 11), and Llufquentue (soil 16) were considered as suppressive against Ggt, since Ggt growth was significantly inhibited when compared with the positive control. However, several soils could not be properly evaluated based on this assay and were classified as undetermined. A second evaluation, using the in vitro inhibition test in aqueous soil extracts (Figure 4B and Supplementary Figure 1B) suggested the presence of nine Ggt-suppressive soils. They were collected from Las Cardas, Momberg, Quilaco, Boyeco, and Llufquentue (soils 2, 3, 4, 6, 11, 13, 14, 15, and 16, respectively). In line with the assay on solid agar, this test also showed that soils collected from Membrillar (soils 7, 9, 10, and 12) were Ggt conducive. This assay also revealed the presence of other Ggt-conducive soils (soils 5 and 8), including the positive control soil 1. In summary, based on in vitro experiments, 9 soils were determined as suppressive, and 7 as conducive (Figure 4B).

Our results on soil chemical properties showed that 25% of the studied soils presented a low content of available P (< 20 mg kg⁻¹), moderate acidity (pH < 5.5), and high Al saturation (>10%), which are main characteristics of agricultural soils from southern Chile (Mora et al., 2006). In general, Andisols grouped together when considering the chemical parameters, whereas Ultisols were more diverse. However, when we compared microbial diversity we observed a direct correlation with soil chemistry mainly in rhizospheric soils, and more significantly for Ultisols. Similar results were found by Smalla et al. (2007) despite the amplified fragments comprised different variable regions and lengths, DGGE, T-RFLP, and SSCP analyses led to clustering of fingerprints, which correlated with soil physico-chemical properties. In Chilean Andisol soils, Jorquera et al. (2014) also showed that soil chemistry influenced the composition of rhizobacterial communities, and in Ultisol soils from China, Li et al. (2017) found through nMDS analyses that microbial communities also correlated with soil chemical parameters and fertilization strategies. Although there is some similarity in microbial composition between rhizosphere and bulk microbial composition (de Ridder-Duine et al., 2005), in our study rhizosphere soils were more diverse in terms of richness and dominance than bulk soils. In fact, it is known that the amount of microorganism around the rhizosphere is 10- to 1,000-fold higher than that found in bulk soil due to rhizodeposition (Doughari, 2015; Glick, 2015).

In terms of potential take-all disease suppression, in vitro Ggt-growth inhibition tests with 16 different soils allowed to identify 9 potentially suppressive soils, and 6 of them were later confirmed to be suppressive in plant bioassays under greenhouse conditions (soil 2, 3, 4, 13, 15, and 16). In general, these soils were cultivated with wheat monoculture and natural pasture for more than 10 years, a management similar to that described previously for other suppressive soils in South Chile (Andrade et al., 2011). Regarding the timing, take-all suppression appeared after 4–6 years of wheat monoculture (McSpadden Gardener and Weller, 2001), and even later, although they can also occur in soils with 3–4 years of monoculture under relatively high pathogen concentrations (Chng et al., 2015). In fact, early studies by Baker and Cook (1974) showed that 3 years of successive wheat cropping could be sufficient for the development of specific suppression. As an exception, soil 2, withrotation based in wheat-triticale and oat for more than 10 years, was also found to be Ggt-suppressive. It is well known that oat roots produce saponin avenacin, a glycosylated triterpenoid secondary metabolite with antifungal properties that has been involved in determining oat resistance to soil fungal pathogens (Osbourn et al., 1994; Freeman and Ward, 2004). On the other hand, wheat plants grown in soil 11, characterized by a very high humidity, showed no symptoms of Ggt infection in roots. This is in agreement with earlier reports by Nish (1973), who studied Ggt survival in the field under controlled conditions, and showed a significant reduction in Ggt incidence in wet cool soils.

In greenhouse assays, wheat plants grown on sterile Ggt-inoculated soils presented the highest disease incidence and the lowest biomass production, suggesting the relevance of the autochthonous soil microbial communities on plant growth promotion and disease suppression. The effect observed in sterile soils—increased susceptibility and reduced biomass—was improved when they were supplemented with 1% of the same natural soils, except in the case of the conducive soils 1 and 14. This improvement also confirms the role of the microbial communities originally present in the take-all disease suppressive soils and Ggt control. This characteristic is known as specific suppression (Cook, 2003; Andrade et al., 2011; Chng et al., 2015). It is noteworthy that we did not find any relation between suppressive soils and the presence of 2,4-DAPG-producing bacteria since its presence was only detected in one out of the six confirmed suppressive soils. The low occurrence of 2,4-DAPG determined by phlD gene, suggests that other mechanism(s) or antifungal compound(s) are synthetized by native soil microorganisms that could contribute to the effective biocontrol against Ggt. Thus, strains related to soil suppressiveness seem to be differentially shaped by multiple soil factors (Imperiali et al., 2017). Therefore, further studies are required to identify the mechanisms involved in Ggt disease suppression.

As mentioned above, the selected suppressive soils did not group together in relation to their chemical properties and geographical origin. However, when bacterial communities were analyzed by DGGE, within Andisols, suppressive soils grouped separately with respect to the control conducive soil 1, but not for Ultisols, in which suppressive soils grouped together with soil 14, also classified as conducive. This could be attributed to the high relation between Ultisol soils and soil chemical parameters when compared to that relation in Andisol soils (r² = 0.90 and 0.59, respectively). Future research should explore which specific microbial groups act directly upon Ggt suppression and how rhizosphere microbial communities are selected and regulated by the plant rhizosphere, especially in the presence of the phytopathogens. Moreover, identifying the bacterial groups and their antagonist mechanisms, as well as exploring the potential stimulation of plant defense mechanisms are pivotal for the development of biocontrol strategies based on the use of suppressive soils. With this aim, future research should tackle the multifactor soil-microbiome-plant-pathogen systems, considering not only direct antifungal activities in the rhizosphere, but also potential stimulation of plant defense and microbe-selection mechanisms.

The authors declare that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest.