Abstract
Background Wheat residues are a crucial determinant of the epidemiology of Septoria tritici blotch, as they support the sexual reproduction of the causal agent Zymoseptoria tritici. We aimed to characterize the effect of infection with this fungal pathogen on the microbial communities present on wheat residues, and to identify microorganisms interacting with it. We used metabarcoding to compare the microbiome associated with wheat residues placed outdoors, with and without preliminary Z. tritici inoculation, comparing a first set of residues in contact with the soil and a second set without contact with the soil, on four sampling dates in two consecutive years.
Results The diversity of the tested conditions, leading to the establishment of different microbial communities according to the origins of the constitutive taxa (plant only, or plant and soil), highlighted the effect of Z. tritici on the wheat residue microbiome. Several microorganisms were affected by Z. tritici infection, even after the disappearance of the pathogen. Linear discriminant analyses and ecological network analyses were combined to describe the communities affected by infection. The number of fungi and bacteria promoted or inhibited by inoculation with Z. tritici decreased over time, and was smaller for residues in contact with the soil. The interactions between the pathogen and other microorganisms appeared to be mostly indirect, despite the strong position of the pathogen as a keystone taxon in networks. Direct interactions with other members of the communities mostly involved fungi, including other wheat pathogens.
Conclusions Our results provide essential information about the alterations to the microbial community in wheat residues induced by the mere presence of a fungal pathogen, and vice versa. Species already described as beneficial or biocontrol agents were found to be affected by pathogen inoculation. The strategy developed here can be viewed as a proof-of-concept for crop residues serving as a particularly rich ecological compartment, with a high diversity of taxa originating from both the plant and soil compartments, and for Z. tritici-wheat as a model pathosystem. By revealing putative antagonistic interactions, we demonstrate that this strategy can be used to improve the biological control of residue-borne diseases.
Background
Septoria tritici blotch (STB) is one of the most important disease of wheat (Triticum aestivum), causing yield losses averaging 20% on susceptible wheat varieties and 5–10% on wheat varieties selected for disease resistance and sprayed with fungicide in Northwestern Europe [1]. It is caused by the hemibiotrophic, heterothallic, ascomycete fungus Zymoseptoria tritici [2], which initiates its sexual reproduction on senescent tissues [3]. STB is clonally propagated between wheat plants during the cropping season by pycnidiospores (asexual spores), which are splash-dispersed upwards over short distances. Wind-dispersed ascospores (sexual spores), mostly produced on wheat residues, initiate subsequent epidemics. Thus, wheat residues are a crucial, but often neglected determinant of the epidemiology of STB during the interepidemic period, as they support the sexual reproduction of the pathogen, maintaining diversity within populations and influencing adaptive dynamics in response to selection pressures [4], through the rapid evolution of fungicide resistance [5–8] or the breakdown of wheat resistance genes [9], for example.
The identification of microorganisms interacting with pathogens is an increasingly important issue for both academic and operational research on the development of biological control solutions [10,11]. In plant, animal and human epidemiology, increasing numbers of studies are trying to characterize variant microbial populations associated with specific disease stages, or temporal changes in the microbial populations during disease progression [12–14]. The pathogen and its cohort of associated microorganisms, which may influence its persistence, transmission and evolution, are together known as the “pathobiome” [15]. Pathobiome research has advanced significantly with the advent of high-throughput sequencing technologies, which have made it possible to describe and follow the diversity of the microbial communities associated with the pathogen during its life cycle, during both the epidemic and interepidemic periods.
The dynamics of microbial communities have been studied in detail during the vegetative and reproductive stages of the plant life cycle, but very few studies during and after plant senescence (e.g. [16,17]). The specific, central position of crop residues in agrosystems was long neglected, but these residues should be seen as both a fully-fledged matrix and a transient compartment: a compartment originating from the plant (temporal link), but in close contact with the soil (spatial link), with variable rates of degradation over the following cropping season, according to the plant species, the cropping practices used, and the climatic conditions in the year concerned [16,19–21]. In addition, the rare studies focusing on the evolution of microbial communities in crop residues performed to date were conducted in microcosms, with sterilized residues (e.g. [22]), in which this compartment is much less complex than under natural conditions.
Several studies have investigated the potential beneficial effects of microorganisms for limiting the development of a plant pathogen during its saprophytic stage on natural crop residues (e.g. Aureobasidium pullulans and Clonostachys rosea inhibiting the sexual stage of Didymella rabiei on chickpea residues [23]; Trichoderma harzianum [24,25], Microsphaerelopsis sp. [26], C. rosea [27,28] and Streptomyces sp. [29] reducing Fusarium graminearum inoculum (perithecia, the sexual fruiting bodies) on wheat or maize residues, as exhaustively summarized in [30]). Other studies have focused on the general impact of cropping practices, such as the increase in microbial soil antagonists induced by the addition of green manure to the soil (e.g. [19,31]). Some phyllosphere microorganisms selected for their antifungal activity against Z. tritici (Bacillus megaterium [32]; Pseudomonas fluorescens [33]; Cryptococcus sp., Rhodotorula rubra and Penicillium lilacinum [34]; T. harzianum [35]; Trichoderma koningii [36]) have been tested in planta against the asexual, pathogenic stage of the pathogen (typically on wheat seedlings), but not against the pathogen during its sexual, saprophytic stage. Moreover, no microbial antagonists of Z. tritici have been isolated from wheat residues, despite the dense population of this habitat with a high diversity of microbial taxa [16].
The taxonomic structure of microbial communities associated with maize [17] and wheat [16] residues has recently been described under natural conditions. In addition to Z. tritici, the microbial communities associated with wheat include Clonostachys sp., Aureobasidium sp., Chaetomium sp. and Cryptococcus sp. [16], all of which are potential competitors. However, the presence of microorganisms in the same ecological niche, as highlighted in such descriptive approaches, does not necessarily mean that interactions actually occur between them. Many other non-interacting microorganisms (pathogens, endophytes) are also present on the residues. Moreover, microbial communities change during the physical degradation of the residues, probably modifying interactions between microorganisms over time [16]. Ecological network analysis has made it possible to detect putative interactions between microorganisms. For instance, Jakuschkin et al. [13] detected significant changes in foliar fungal and bacterial communities following the infection of pedunculate oak with Ersysiphe alphitoides (the causal agent of oak powdery mildew), and Cobo-Diaz et al. [17] identified candidate antagonists of toxigenic Fusarium spp. among the species present in maize residues. The use of co-occurrence networks in these two studies highlighted a set of bacteria and fungi that might be useful for managing plant pathogens.
In this study, our goal was to identify fungi and bacteria potentially interacting with Z. tritici during its sexual reproduction on wheat residues. To this end, we compared the structure of microbial communities associated with wheat residues with and without Z. tritici inoculation, by metabarcoding, combining linear discriminant analyses (LDA) and ecological network analyses. The response of microbial communities to Z. tritici infection was assessed during the interepidemic period between two successive crops, for two sets of wheat residues, one left outdoors in contact with the soil, and the other left outside but not in contact with the soil, at different sampling dates during two consecutive years. The diversity of experimental conditions was expected to lead to the establishment of different microbial communities according to the origin of the constitutive taxa (plant or soil), thereby increasing the probability of detecting effects of Z. tritici on the residue microbiome, and of the residue microbiome on Z. tritici.
Results
Overall diversity of the bacterial and fungal communities on residues
The response of the residue microbiome to Z. tritici inoculation was assessed by analyzing the composition of the fungal and bacterial communities of wheat residues, after inoculation with Z. tritici (n=240) or in the absence of inoculation (n=240). We also investigated the impact of cropping season (n=2), season (n=4), and soil contact (n=2) on the dynamics of these communities (see materials and methods for a detailed explanation of the experimental design; Figure 1).
We investigated the structure of the residue microbiome by analyzing the v4 region of the 16S rRNA gene and ITS1. Overall, 996 bacterial amplicon sequence variants (ASVs) and 520 fungal ASVs were obtained from 390 and 420 samples, respectively. Some samples (July 2016) were removed from the analysis due to the co-amplification of chloroplasts.
The high relative abundance (RA) of ASVs affiliated to Z. tritici in samples collected in July 2016 (21.5±9.8%) and 2017 (30.3±7.1%) highlights successful colonization of the wheat tissues by this pathogen following inoculation (Figure 2). However, the RA of Z. tritici rapidly decreased to 2±1.64% and 1.4±0.9% on residues not in contact with the soil (“above ground” residues) collected in October 2016 and 2017, respectively, and this species was below the limit of detection in December and February. For residues in contact with soil, this decrease occurred more rapidly, with Z. tritici already undetectable in samples collected in October.
Alpha diversity, estimated with the Shannon index, was low in July for both bacterial (2.70±0.75) and fungal communities (1.82±0.19; Suppl. Figure 1). A gradual increase was then observed during residue degradation. Z. tritici inoculation had no impact on bacterial alpha-diversity, but decreased fungal diversity (Kruskal-Wallis: p = 0.008). More specifically, bacterial diversity was higher in inoculated residue samples in July 2017 (2.92±0.80 for inoculated samples versus 2.47±0.6 for non-inoculated samples; Wilcoxon: p = 0.022), but no such difference was detected for the other sampling dates. Conversely, for fungal communities, inoculation had no effect in July, but led to a significant decrease in diversity in subsequent months during the second cropping season (October and December 2017, for the two soil contact conditions).
Beta diversity analysis (Bray-Curtis index) showed large dissimilarities between bacterial community composition in July and at the other sampling dates, as illustrated in the hierarchical clustering of the samples, justifying separate analyses and MDS representations (Figure 3). Inoculation with Z. tritici had a minor effect on bacterial communities, with only 5% of the variance explained for samples collected in July (PERMANOVA: p = 0.004). By contrast, in the same month, inoculation was the structuring factor for fungal communities, accounting for 33% of the variance (PERMANOVA: p = 0.001). For subsequent samplings (October, December and February), temporal conditions (seasonality and cropping season) were the main factors influencing fungal communities. Soil contact was the main structuring factor for bacterial communities, with a stronger effect than seasonality or cropping season (Table 1).
Impact of contact with the soil on microbial communities
The significant impact of soil contact on microbial communities highlighted differences in the process of wheat residue colonization. MDS analysis suggested that the communities of “above ground” residue samples collected in October were less different from those collected in July than from the communities of “soil contact” samples also collected in October (Figure 4). Contact with the soil, therefore, caused a greater change in communities, suggesting competition between plant-associated taxa and soil-borne taxa. Taxonomic differences between the communities present on residues in contact with the soil and those present in above ground residues were highlighted in linear discriminant analysis (LDA).
Some classes of taxa (e.g. Bacilli, Sphingobacteria, Betaproteobacteria, Dothideomycetes, Pezizomycetes) were particularly abundant only in above ground residues, suggesting that they were mostly derived from the plant. By contrast, other classes (e.g. Alphaproteobacteria, Agaricomycetes, Cytophagia, Gammaproteobacteria) were more prevalent in residues in contact with soil, suggesting that they originated from the soil (Suppl. Figure 2). The abundance of some classes varied with cropping season (e.g. Flavobacteria). Soil contact had a large impact for Dothideomycetes and Bacilli, which were highly abundant in July, but rapidly decreased in frequency when the residues were in contact with the soil. Pezizomycetes, absent in July, colonized only the above ground residues. Conversely, the percentage of reads associated with Alphaproteobacteria, which was quite high in July, and Cytophagia, which was low in July, increased over time, particularly in residues in contact with the soil. Similarly, Agarycomycetes, which was completely absent in July, colonized only residues in contact with the soil.
At the genus level, 87 (excluding “unclassified”) of the 273 genera (60/190 for bacteria; 27/83 for fungi) identified displayed differences in abundance between above ground residues and residues in contact with the soil, for at least one date (Figure 4). For example, Bosea, Rhizobium, Nocardioides, Pseudomonas, and Sphingomonas were more abundant in residues in contact with the soil, whereas Cladosporium, Massilia, Paracoccus, Stagonospora and Cryptococcus were more abundant in above ground residues.
Impact of Z. tritici inoculation on microbial communities
The influence of Z. tritici on the RA of residue microbiome members was assessed, through LDA scores. In total, the RA of 115 ASVs (74 bacterial ASVs and 41 fungal ASVs) was significantly affected by Z. tritici inoculation, for at least one sampling date (listed in Suppl. Figure 3). The effect of inoculation on microbial communities persisted throughout the experiment, despite the absence of Z. tritici detection from December onwards (Figure 2). ASVs with significant differences in RA decreased over time for residues in contact with the soil (Suppl. Table 1). By contrast, for above ground residues, the number of differential ASVs increased until December, in both cropping seasons (20 ASVs in December 2016-2017; 31 ASVs in December 2017-2018).
Inoculation with Z. tritici decreased the number of fungal ASVs, including those affiliated to Sarocladium, Gibellulopsis and Blumeria, and increased the number of bacterial ASVs affiliated to Curtobacterium and Brachybacterium (listed in Suppl. Figure 3). The ASVs affected by inoculation differed between above ground residues and residues in contact with soil. The pattern of change (i.e. promoted or inhibited by inoculation) was always the same within a given year, regardless of soil contact conditions. For example, Brachybacterium and Curtobacterium were promoted by inoculation, in both soil contact conditions, whereas Sarocladium was inhibited by inoculation, in both soil contact conditions.
Impact of the actual presence of Z. tritici on microbial communities
Microbial analysis networks combining bacterial and fungal datasets were used to predict the potential interactions between Z. tritici and members of microbial communities associated with wheat residues.
Dynamics of ecological interaction networks
The dataset was split according to the effects previously described (cropping season, seasonality, soil contact conditions). Six ecological interaction networks were generated per experimental year, corresponding to residue samples in contact with the soil and above ground residues, collected in October, December, and February (Figure 5). The networks for July are presented in Suppl. Figure 4. The mean number of nodes in the network (205.3±47.5) increased over the season (Suppl. Table 1). Overall, networks were very sparse, with a mean node degree of 2.76±0.43. For each network, the positive/negative edge ratio decreased over time, reaching 1.0-1.5 in February. Most nodes were common to October, December and February. Z. tritici was one of the fungi with the largest number of degrees and greatest betweenness (measurement of centrality in a graph based on the shortest paths) for above ground samples in October. By contrast, for samples in contact with soil, it was absent the first year and had low betweenness and degree values for the second year (Figure 6).
Subnetworks highlighting direct interactions between Z. tritici and other microorganisms
Ecological interaction networks were combined with LDA to investigate the interactions between Z. tritici and members of the microbial communities of residues (Figure 7). Only 13 of the 115 ASVs affected by inoculation (LDA) were in direct interaction with Z. tritici, indicating an indirect effect of Z. tritici on the community (no direct connection between the microorganisms).
Microorganisms with the same differential pattern (i.e. “promoted by inoculation” or “promoted in the absence of inoculation”) did not interact negatively with each other in networks. Conversely, microorganisms with opposite differential patterns systematically interacted negatively with each other. These results highlight the consistency of the LDA and ecological interaction network analysis approaches.
The subnetworks generated with microorganisms presenting differential relative abundances and their adjacent nodes were strongly connected: each subnetwork consisted of a principal component and, in some cases, smaller components of less than four nodes (Figure 7).
Only a few direct interactions between Z. tritici and other microorganisms were highlighted in ecological interaction networks. Some ASVs affiliated to the same genus had opposite interaction trends with Z. tritici, such as Fusarium ASVs in July 2017, or Cladosporium ASVs in October 2016, consistent with the findings of LDA analyses. In some cases, the same ASV had different interaction trends at different sampling dates or in different years. This was the case for Acremonium ASVs (negative interaction in October 2016, positive interaction in October 2017). Some genera, such as Blumeria, Sarocladium, and Penicillium, interacted only negatively with Z. tritici. Symmetrospora, Brachybacterium, and Monographella interacted only positively with Z. tritici.
Discussion
By sequencing the microbial communities of 420 samples of wheat residues, we obtained a total of 996 bacterial ASVs and 520 fungal ASVs. Using this large dataset, we estimated the potential interactions occurring between a plant pathogen (Z. tritici) and the members of microbial communities associated with crop residues in field conditions. By combining two approaches — LDA and network analysis — we were able to demonstrate an effect of pathogen infection, even after disappearance of the pathogen, on the structure and composition of the microbial communities during residue degradation.
Effect of soil contact on microbial communities
Our aim here was not to characterize the organisms colonizing wheat residues, but our findings nevertheless highlight major changes in the microbial community over time for residues in contact with soil. The taxa favored in above ground residues, such as Cladosporium, Alternaria, Pedobacter and Massilia, were already present on the plant. This is consistent with previous findings showing a decrease in the abundance of these plant-associated taxa during the degradation of residues in contact with soil and the colonization of these residues with soil-borne competitors, such as Chaetomium, Torula, and Nocardioides [16]. Some fungal genera not present in July were favored by above ground conditions (e.g. Cryptococcus, Stagonospora, and Myrmecridium). This finding is consistent with our knowledge of fungal dispersal processes, mostly involving aerial spores.
Disappearance of Z. tritici during residue degradation
Z. tritici rapidly disappeared between October and December. This finding is surprising in light of the quantitative epidemiological data acquired for the same plot, which suggested that Z. tritici ascospores may be ejected from residues until March [3,37]. The observed disappearance of Z. tritici may be due to lower levels of contamination of adult wheat plants in residues than would be achieved in the field after natural infection. Indeed, in field conditions, Z. tritici establishes itself on all parts of the plant (leaves, but also sheaths and stems) through multiple secondary infections, driven by the repeated splash dispersal of asexual spores, leading to an accumulation of contaminating raindrops at the points of insertion of the leaf sheaths. The single inoculation event in the greenhouse resulted in contamination principally of the leaves, the organs most exposed to spraying, with relatively little contamination of the stems and sheaths, the parts of the plant most resistant to degradation. Indeed, the results of a previous study [16] support this hypothesis: in the same field, during the same season, Z. tritici was detected in wheat residues originating from plants grown in natural conditions until February, and even May, with a similar metabarcoding approach.
Effect of Z. tritici on microbial communities
Endophytes and pathogens induce changes in plant tissues (e.g. necrosis), which may themselves modify the microbial communities inhabiting the plant (e.g. impact of secondary saprophytes or opportunistic pathogens [38]; selection of microorganisms by secondary metabolites produced by microorganisms or the plant; [39,40]). This general phenomenon may explain the impact of Z. tritici on the microbial communities observed in both LDA and network analysis. The impact of Z. tritici on residues, even after its disappearance between October and December, persisted until February, particularly for fungal communities. Within microbial networks, Z. tritici was one of the keystone taxa, despite its low abundance, in above ground residues in October (Suppl. Figure 5). The high levels of Z. tritici in July (between 10 and 40% of reads) account for its central position in the network. The number of microorganisms displaying changes in abundance due to Z. tritici inoculation decreased during residue degradation. This finding highlights the resilience of the community (i.e. its ability to return to its original composition after a disturbance, in this case, Z. tritici inoculation) [41].
Specific interactions with Z. tritici
Most of the predicted interactions with Z. tritici involved fungi, such as Fusarium, Blumeria or Cladosporium. Z. tritici infection has been shown to be associated with the accumulation of H2O2 [42]. This compound is known to inhibit biotroph fungal pathogens [43], such as Blumeria graminis [44,45]. This may explain the negative interaction between Z. tritici and B. graminis in July and October 2017-2018. In addition, Z. tritici infection induces leaf necrosis, potentially decreasing wheat susceptibility to B. graminis, due to a significant physiological interaction during the latent, endophytic period of Z. tritici development [45]. H2O2 is also known to promote necrotrophic agents, such as Fusarium. We detected both positive and negative interactions between Z. tritici and Fusarium, depending on the ASV considered. On adult wheat plants, such differential interactions have been demonstrated in log-linear analyses [46], with both species giving positive results on stem bases and negative results on the upper parts of stems. Positive interactions between Z. tritici and Cladosporium have also been demonstrated on adult plants [46], consistent with our findings for wheat residues. These results lend a biological meaning to the interactions detected, confirming the relevance of network analyses for highlighting ecological interactions within crop residue communities.
Trichoderma was more abundant in residues from wheat plants inoculated with Z. tritici (July 2016), as shown by LDA (Suppl. Figure 4). Conversely, Epicoccum and Cryptococcus were more abundant in residues from non-inoculated wheat plants (October 2016). The overabundance of those taxa, described as biocontrol agents in previous studies [34–36,47], was influenced by the presence of the pathogen. However, no direct interactions between Z. tritici and these species could be established. This exemplifies the difficulties highlighting beneficial species within complete microbial communities. These difficulties are not specific to the residue compartment and also apply to the spermosphere [48], phyllosphere [49] and rhizosphere compartments [14,50].
Other interactions
Other interactions between ASVs highlighted in the network analysis were examined in light of published results for fungal pathogens of cereals. For instance, it has already been shown that B. graminis growth on barley is inhibited by Trichoderma harzianum [51] and Stagonospora norodum [52], that Stenetrophomas maltophila attenuates the seedling blight of wheat caused by F. graminearum [53], that Acremonium zeae has antibiotic activity against Fusarium verticillioides [54], and that Chaetomium sp. produces compounds (e.g. chaetomin) active against Alternaria triticimaculans [34]. Conversely, certain non-pathogenic bacteria were shown to be associated with significantly more disease on wheat caused by B. graminis and Z. tritici and to “help” Phaeosphaeria nodorum to infect wheat tissues [55]. Newtoon et al. [38] has proposed the hypothesis of “induced susceptibility” to explain such an interaction between bacteria and biotroph fungal pathogens.
The analysis of ecological network also suggested that intra-kingdom interactions were favoured over inter-kingdom interactions in certain conditions (Suppl. Table 2). This may reflect differences in ecological niches and dynamics, as illustrated by the temporal changes in microbial communities over a season, with a densification of the networks during residue degradation. Further investigations are required to determine whether inter- or intra-kingdom interactions are more intense, and thus more promising for use in biocontrol engineering. Should we preferentially focus on fungal communities to improve the management of a fungal disease, and on bacterial communities to improve the management of a bacterial disease?
Identification of beneficial species, and potential biocontrol agents
Network models provide new opportunities for enhancing disease management and can be helpful for biocontrol. Our study, combining LDA and ecological network analyses based on a metabarcoding approach and differential conditions (plants inoculated with a pathogen or left non-inoculated; plant residues in contact with soil vs. residues not in contact with the soil), fits into the framework described by Poudel et al. [56], which considers several types of network analyses, including pathogen-focused analyses, taking into account diseased and healthy plant hosts, with a view to elucidating direct and indirect pathogen-focused interactions within the pathobiome.
Network analyses revealed no significant direct interactions between Z. tritici and microorganisms reported to be useful biocontrol agents. However, pathogen infection had a strong effect on the entire microbial community present in residues during the course of their degradation. Most of the interactions were difficult to interpret. Several interactions appeared to be transient, changing over time with residue degradation, and their presence or absence depended on whether the residues were in contact with the soil. This suggests that interactions between microorganisms are not very stable, and can be modified by changes in the environment, for example, or by the arrival of a new microorganism.
The neglect of complex interactions between biocontrol agents and their biotic environment (the plant, the soil and their microbiomes), the physical and chemical properties of which change over time, may account for lower levels of efficacy in field conditions than in laboratory conditions (concerning the phyllosphere, e.g. [38], but also the residue compartment, e.g. [57]). Indeed, several studies have demonstrated the value of studying the effect of entire communities on biotic and abiotic stresses rather than the effects of single species. For example, resistance to B. cinerea in Arabidopsis thaliana was shown to be not due to a single species, but to the action of the microbiome as a whole [58]. By comparing the structure of microbial communities associated with Brassica rapa plants inoculated with the root pathogen Plasmodiophora brassicae, Lebreton et al. [14] showed significant shifts in the temporal dynamics of the root and rhizosphere microbiome communities during root infection. Moreover, the rhizospheres of plants infected with P. brassicae were significantly more frequently colonized with a Chytridiomycota fungus, suggesting interactions between these two microorganisms.
The most frequently studied cases of microbial community effects include “suppressive soils”, which provide defense against soil-borne pathogens, rendering them unable to establish themselves or to persist in the soil or the plant [59]. The basis and dynamics of this disease suppression vary, and suppression may be general or specific, under the control of antibiotic-producing Pseudomonas or Streptomyces populations, for example [60]. Differences in the composition, structure and diversity of microbial communities on crop residues remain poorly understood, and further studies are required to determine the potential for use in biocontrol not of single agents, but of microbial communities, as for these suppressive soils. Despite this ecological reality, the current perception of biocontrol engineering is still too often limited to the action of a single species, even a single strain, with a direct, strong and durable effect against a plant pathogen.
Potential utility of the residue microbiome
Improving our understanding of the relationship between biodiversity and ecosystem functioning will require the development of methods integrating microorganisms into the framework of ecological networks. Exhaustive descriptions of microbial diversity combined with network analysis are particularly useful for identifying species within microbial communities of potential benefit for disease management [56]. By revealing antagonistic interactions between pathogen species (e.g. Z. tritici) and other microorganisms, our study suggests that this strategy could potentially improve the control of residue-borne diseases, as suggested by another recent study on Fusarium [17]. This strategy, which has been developed separately for the plant [61,62] and soil [14,50,63] compartments, would undoubtedly benefit from further development on crop residues. Indeed, decreasing the presence of pathogens on residues during the interepidemic period can decrease disease development on subsequent crops [21]. The strategy developed here can be viewed as a proof-of-concept for the use of crop residues as a particularly rich ecological compartment containing a high diversity of taxa originating from both the plant and soil compartments, and for the use of Z. tritici-wheat as a model pathosystem. Understanding the complex interactions between a pathogen, crop residues and other microbiome components in the shaping of a plant-protective microbiome is essential, to improve the efficacy of biocontrol agents and to preserve existing beneficial equilibria through the adoption of appropriate agricultural practices.
Methods
We investigated the effect of Z. tritici on the diversity of the wheat microbiome and the effect of the wheat microbiome on Z. tritici, by characterizing the composition of the microbial communities of 420 residue samples (210 per year) from plants with and without preliminary Z. tritici inoculation. The residues were placed outdoors, either directly in contact with the soil in a field plot or “above ground”, i.e. not in contact with the soil, to assess the effect of their colonization by microorganisms originating from the soil, the plant and the air on the saprophytic development of Z. tritici. We investigated the persistence of interactions between the pathogen and the whole microbial community, and changes in those interactions over time, by sampling the residues before exposure to outdoor conditions (in July), and every two months thereafter (in October, December, and February) (Figure 1).
Preparation of wheat residues
The 420 wheat residue samples were obtained from 60 winter wheat cv. Soissons plants grown in a greenhouse in each of the two years of the study, as described in [64]: two weeks after sowing, seedlings were vernalized for eight weeks in a growth chamber and then transplanted into pots. Three stems per plant were retained. Half the wheat plants were inoculated with a mixture of four Z. tritici isolates (two Mat1.1. isolates and two Mat1.2 isolates; [65]) to ensure that sexual reproduction occurred as in natural conditions. This equiproportional conidial suspension was prepared and adjusted to a concentration of 2 × 105 spores.mL-1, as previously described [64]. Thirty plants were inoculated at the late heading stage in early May, by spraying with 10 mL of inoculum suspension. The other thirty plants were sprayed with water, as a control. Inoculated and non-inoculated plants were enclosed in transparent plastic bags for three days to ensure moist conditions favoring pathogen infection. Septoria tritici blotch lesions appeared three to four weeks after inoculation (Figure 1A). All plants were kept in the same greenhouse compartment until they reached complete maturity (mid-July).
For each “inoculated” and “non-inoculated” condition, stems and leaves were cut into 2 cm-long pieces and homogenized to generate the “wheat residues”, which were then distributed in 105 nylon bags (1.4 g per bag; Figure 1B) for each set of inoculation conditions, in each year.
Exposure of residues to natural conditions
Ninety nylon bags were deposited in contact with the soil in a field plot (the “soil contact” treatment) or without contact with the soil (“above ground” residue treatment). Thirty batches of residues (15 inoculated and 15 non-inoculated) were used to characterize the communities present in July before the exposure of the residues in the nylon bags to natural conditions. The field plot (“OWO” in [16]; Grignon experimental station, Yvelines, France; 48°51′N, 1°58′E) was the same in both cropping seasons. It was sown with wheat in 2015-2016, with oilseed rape in 2016-2017, and with wheat in 2017-2018. The 90 bags for the “soil contact” treatment were deposited in the OWO field plot (Figure 1C) in late July, at 15 sampling points 20 m apart (three “inoculated” and three “non-inoculated” bags at each sampling point). The 90 bags of the “above ground” treatment were placed on plastic grids exposed to outdoor conditions and located about 300 m from the OWO field plot (Figure 1D).
We assessed the impact of seasonality on the fungal and bacterial communities on residues by collecting samples of each “inoculated” and “non-inoculated” treatment at three dates (October, December and February): 15 bags from plastic grids (“above ground” treatment) and one bag from each sampling point in the field (“soil contact” treatment) At each date, nylon bags were opened, the residues were rinsed with water and air-dried in laboratory conditions. Residues were then crushed with a Retsch™ Mixer Mill MM 400 for 60 seconds at 30Hz with liquid nitrogen in a Zirconium oxide blender.
Total DNA extraction
Total DNA was extracted with the DNeasy Plant Mini kit (Qiagen, France), with a slightly modified version of the protocol recommended by the manufacturer. Powdered residues (20 mg), 450 µL of Buffer AP1 preheated to 60°C, RNase A and Reagent DX (450: 1: 1) were mixed vigorously for 15 s in a 2 mL Eppendorf tube. Buffer P3 (130 µL) was added to each tube, which was then shaken manually for 15 s, incubated at −20°C, and centrifuged (1 min, 5000 g). The supernatant (450 µL) was transferred to a spin column and centrifuged (2 min, 20000 g). The filtrate (200 µL) was transferred to a new tube, to which sodium acetate (200 µL, 3 M, pH 5) and cold 2-propanol (600 µL) were added. DNA was precipitated by incubation at −20°C for 30 min and recovered by centrifugation (20 min, 13000 g). The pellet was washed with cold ethanol (70%), dried, and dissolved in 50 µL of AE buffer.
PCR and Illumina sequencing
Fungal and bacterial communitiesprofiles were analyzed by amplifying ITS1 and the v4 region of the 16S rRNA gene, respectively. Amplifications were performed with ITS1F/ITS2 [66] and 515f/806r [67] primers. All PCRs were run in a total volume of 50 µL, with 1x Qiagen Type-it Multiplex PCR Master Mix (Type-it® Microsatellite PCR kit Cat No./ID: 206243), 0.2 µM of each primer, 1x Q-solution® and 1 μl DNA (approximately 100 ng). The PCR mixture was heated at 95°C for 5 minutes and then subjected to 35 cycles of amplification [95°C (1 min), 60°C (1 min 30 s), 72°C (1 min)] and a final extension step at 72°C (10 min). PCR products were purified with Agencourt® AMPure® XP (Agencourt Bioscience Corp., Beverly, MA). A second round of amplification was performed with 5 μl of purified amplicons and primers containing Illumina adapters and indices. PCR mixtures were heated at 94°C for 1 min, and then subjected to 12 cycles of amplification [94°C (1 min), 55°C (1 min), 68°C (1 min)] and a final extension step at 68°C (10 min). PCR products were purified and quantified with Invitrogen QuantIT™ PicoGreen®. Purified amplicons were pooled in equimolar concentrations, and the final concentration of the library was determined with the qPCR NGS library quantification kit (Agilent). Libraries were sequenced in four independent runs with MiSeq reagent kit v3 (600 cycles).
Sequence processing
Runs were analyzed separately. Primer sequences were first cut off in the fastq files with Cutadapt [68]. Files were then processed with DADA2 v.1.8.0 [69] according to the recommendations for the “DADA2 Pipeline Tutorial (1.8)” workflow [70], with quality trimming adapted for each run (Suppl. Table 3).
A mock sample consisting of equimolar amounts of DNA from known microorganisms was included in each run (see Suppl. Figure 6) to establish a detection threshold for spurious haplotypes. At a threshold of ≤ 0.3 ‰ of the size of the library, amplicon sequence variants (ASVs) were considered spurious and were removed from the sample. We used the naive Bayesian classifier on RDP trainset 14 [71] and the UNITE 7.1 database [72] to assign ASVs. ASVs as assigned to chloroplasts (for bacteria) or unclassified at the phylum level (for bacteria and fungi) were also removed from each sample. Due to large proportion of chloroplast sequences among the 16S rRNA gene products, all samples from July 2017 were removed from the analysis.
Differential community analysis
For microbial community analyses, the total library size of each sample was standardized by normalization by proportion. The experimental conditions taken into account were cropping season (2016-2017 and 2017-2018), seasonality (four sampling dates: July, October, December, and February), inoculation with Z. tritici (inoculated and non-inoculated), soil contact (soil contact and above ground treatments). The Shannon diversity index was used to assess the effect of each set of conditions on fungal and bacterial diversity. The divergence of microbial communities between samples was assessed by calculating the Bray-Curtis dissimilarity matrix with the phyloseq package (v 1.24.2 [73]), and then illustrated by MDS and clustering based on the average linkage method (ape package v 5.2. [74]). PERMANOVA was performed with the “margin” option, to test the effect of each factor on communities (adonis2 function, vegan package [75]).
A linear discriminant analysis (LDA) implemented in Galaxy [76] (LefSe, http://huttenhower.org/galaxy) was used to characterize the differential abundances of fungal and bacterial taxa between each soil contact condition and each Z. tritici inoculation condition. In this analysis, differences in the relative abundance of taxa between treatments were evaluated with a Kruskal-Wallis test; a Wilcoxon test was used to check, by pairwise comparisons, whether all subclasses agreed with the trend identified in the Kruskal-Wallis test. The results were used to construct an LDA model, to discriminate between taxa in the different conditions. For the comparison between “soil contact” and “above ground” treatments, inoculation condition was used as a subclass, with the Wilcoxon test alpha value set at 0.05, and the alpha value of the Kruskal-Wallis test set at 0.01. For the comparison between “inoculated” and “non-inoculated” treatments, the alpha value of the Kruskal Wallis test was set at 0.01 (no subclasses). For both analyses, the threshold for the LDA analysis score was set at 2.0.
Ecological interaction network analyses
For characterization of interactions within the different wheat residue microbial communities, we used ecological interactions networks calculated with SPIEC-EASI [77] for combined bacterial and fungal datasets [78]. The same parameters were used for all networks. The non-normalized abundance dataset was split on the basis of sampling date and soil contact condition. Each of the datasets included 30 samples (15 inoculated samples and 15 non-inoculated samples). Infrequent ASVs were filtered out by defining a threshold of a minimum of six occurrences. We used the neighborhood selection as graphical inference model (Meinshausen and Bühlmann MB method) with SPIEC-EASI, as this method has been shown to outperform most of the other available methods (e.g. CCREPE, SPARCC, SPIEC-EASI (glasso)) [77]. The StARS variability threshold was set at 0.05. Networks were then analyzed with the igraph package (version 1.2.2. [79]). Scripts for network construction and analysis are available from GitHub (see Availability of data and materials).
Subnetworks for analysis of the Z. tritici pathobiome
We used a dual approach to characterize interactions between Z. tritici and the other taxa, based on: (i) the LDA scores obtained in differential analyses between Z. tritici inoculation conditions (“inoculated” and “non-inoculated” treatments); (ii) ecological network analysis. LDA identified taxa affected by inoculation conditions (definition of classes for samples) and network analysis identified interactions at the sample scale (without prior assumptions). Subnetworks of differential ASVs and their adjacent nodes were established by combining these two approaches. Subnetworks were visualized with Cytoscape V. 3.6.1 [80]
Funding
This study was supported by a grant from the European Union Horizon Framework 2020 Program (EMPHASIS Project, Grant Agreement no. 634179) covering the 2015-2019 period.
Availability of data and materials
The raw sequencing data are available from the European Nucleotide Archive (ENA) under study accession number PRJEB31818. We provide the command-line script for data analysis and all necessary input files via GitHub (https://github.com/LydieKerdraon/MicrobialNetworkAnalysis-WheatResidues).
Authors’ contributions
LK, FS, VL, MB conceived the study, participated in its design, and wrote the manuscript. LK conducted the experiments and analyzed the data. FS and VL supervised the project. All authors read and approved the final manuscript.
Ethics approval and consent to participate
Not applicable
Consent for publication
Not applicable
Competing interests
The authors declare that they have no competing interests.
Acknowledgments
This study was performed in collaboration with the GeT core facility, Toulouse, France (http://get.genotoul.fr/), supported by France Génomique National Infrastructure, funded as part of the “Investissement d’avenir” program managed by Agence Nationale pour la Recherche (contract ANR-10-INBS-09). We thank Angelique Gautier for preparing the mocks, Nathalie Retout (INRA BIOGER) and Christophe Montagnier (INRA Experimental Unit, Thiverval-Grignon) for technical assistance, Anne-Lise Boixel (INRA BIOGER) for assistance with statistical analyses, and Marie-Hélène Balesdent (INRA, UMR BIOGER) for her comments and suggestions to improve the manuscript. We thank Julie Sappa for her help correcting our English.
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