Assessing the responses of Sphagnum micro-eukaryotes to climate changes using high throughput sequencing

Current projections suggest that climate warming will be accompanied by more frequent and severe drought events. Peatlands store ca. one third of the world’s soil organic carbon. Warming and drought may cause peatlands to become carbon sources through stimulation of microbial activity increasing ecosystem respiration, with positive feedback effect on global warming. Micro-eukaryotes play a key role in the carbon cycle through food web interactions and therefore, alterations in their community structure and diversity may affect ecosystem functioning and could reflect these changes. We assessed the diversity and community composition of Sphagnum-associated eukaryotic microorganisms inhabiting peatlands and their response to experimental drought and warming using high throughput sequencing of environmental DNA. Under drier conditions, micro-eukaryotic diversity decreased, the relative abundance of autotrophs increased and that of osmotrophs (including Fungi and Peronosporomycetes) decreased. Furthermore, we identified climate change indicators that could be used as early indicators of change in peatland microbial communities and ecosystem functioning. The changes we observed indicate a shift towards a more “terrestrial” community in response to drought, in line with observed changes in the functioning of the ecosystem.


INTRODUCTION
Although much remains to be done before we can fully predict future climate variability (Ljungqvist et al., 2016), current projections suggest that climate warming will be accompanied by more frequent and severe drought events (Dai, 2013) thus affecting terrestrial communities. Amongst these, eukaryotic micro-organisms play key roles in ecosystem functioning as primary producers, decomposers predators and parasites (e.g., Fell et al., 2006;Geisen et al., 2018;Jassey et al., 2013a). Alterations in microeukaryotic community structure and diversity caused by ongoing environmental changes, including global warming and drought, may affect ecosystem functioning (Arndt & Monsonís Nomdedeu, 2016;Petchey et al., 1999), making it all the more necessary to include micro-eukaryotes in climate change studies (Cavicchioli et al. (2019).
Peatlands store one third of the world's soil organic carbon (i.e., 500 ±100 GtC; Yu, 2012), but are particularly sensitive to climate induced perturbations, threatening their role in the C-cycle. Indeed, warming accompanied by drought which stimulates microbial activity (Bardgett, Freeman & Ostle, 2008;Freixa et al., 2017) leads to disruption of the peatlands' function as C sinks and turns these ecosystems into carbon sources through increased respiration (Dorrepaal et al., 2009), with positive feedback effect on warming (Baird et al., 2013;Davidson & Janssens, 2006;Gorham, 1991;Yu, 2012). Peatland carbon balance is controlled by primary production (mainly by plants, to a lesser extent by autotrophic and mixotrophic micro-organisms; Jassey et al. (2015)) and decomposition (mainly by bacteria and fungi). Microbial activity is increased by micro-eukaryotic grazing on bacteria and fungi (e.g., Hahn & Höfle, 2001), implying that the standing biomass of bacteria and fungi does not necessarily correlate to decomposition intensity and their turnover may be enhanced under warmer or drier conditions. Therefore, identifying the factors that influence micro-eukaryotic community structure and diversity is crucial for our understanding of potential peatland feedbacks on climate warming.
The significance of peatlands in the global C cycle is in large part due to the unique biological characteristics of Sphagnum mosses, the main builders of high latitude peatlands. Sphagnum mosses are adapted to acidic, water-logged and nutrient-poor conditions, which they contribute to create (Rydin, Jeglum & Hooijer, 2006). Clymo & Hayward (1982) suggested that more C might be stored in Sphagnum (living and dead) than in any other plant genus. Sphagnum and its associated specific microbial community constitutes a microecosystem called ''sphagnosphere'' and this complex system may be the key to the nutrient cycling in peatlands (Chiapusio et al., 2013), and hence to its C-sequestrating function. Sphagnum-associated microbial communities change in composition and also functionally along climatic (Singer et al., 2019) and micro-environmental gradients (Mitchell et al., 2003). The Sphagnum microbiome may supports its host through nutrient supply and defence against pathogens (Bragina et al., 2013;Raghoebarsing et al., 2005), and ultimately the ecosystem under changing climate (Bragina et al., 2014).
Warming has indirect effects on microbial food web structure, altering the community composition and ecosystem functioning (Jassey et al., 2011). For instance, Tsyganov et al. (2012 have shown that the response to climate change differs among seasons, and that testate amoebae, a dominant group of microbial top predators in peatlands (Gilbert et al., 1998;Jassey et al., 2013b;Jassey et al., 2012;Meyer et al., 2013;Mieczan, 2007) are especially sensitive during the growing season. Tveit et al. (2015) showed that warming caused an increase in the relative abundance of Cercozoans (phagotrophic protists), higher substrate turnover and microbial activity as well as changes in methanogenic pathways. Jassey et al. (2013a) demonstrated that warming reduced the abundance of top predators while the biomass of bacteria increased. Such changes in microbial community structure can potentially alter the above-belowground linkages, destabilizing the C cycle (Jassey et al., 2013a).
Peatlands are particularly sensitive to drought, as these ecosystems are primarily controlled by the high water level that creates anoxic conditions allowing peat to accumulate. Indeed, severe drought might induce changes in peatland ecosystem function, turning them into carbon sources (Jassey et al., 2018). Drought alters community composition (Potter et al., 2017), shifting the community towards species adapted to dry habitats (Koenig, Mulot & Mitchell, 2018). Prolonged drought conditions might lead to loss of key species or decrease their abundance below the level necessary to drive ecosystem function (Jenkins & Boulton, 2007). The resulting destabilization of the food-web structure might then cross a tipping point and shift the C balance (Dakos et al., 2019;Lamentowicz et al., 2019).
The goal of this study was to assess the diversity and community composition of eukaryotic microorganisms inhabiting Sphagnum in peatlands, with a main focus on protist communities, and their response to experimental drought and warming. We hypothesized that (1) the diversity and community structure of micro-eukaryotes vary in response to drought and warming. More specifically, we hypothesised that (2) drought causes a decrease in the relative abundance and diversity of primary producers, as microalgae predominantly inhabit aquatic environments (e.g., Ray et al., 2019), (3) an increase in the diversity and relative proportion of fungi, as it has been suggested that drought leads to increased dominance of fungi (Jensen et al., 2003), and this agrees with observational evidence for a higher contribution of fungi to overall microbial biomass under drier conditions (Mitchell et al., 2003), although responses might be site-specific (Jaatinen et al., 2007); (4) the effects of drought are exacerbated by the effects of warming; and (5) drought has a stronger effect than warming. To this aim, we conducted a passive warming and water table depth field manipulative experiment and assessed the diversity of micro-eukaryotes by high throughput sequencing (Illumina HiSeq) of the SSU rRNA V9 region.

Study site and field experiment
The study site, Linje peatland (53 • 11 15 N, 18 • 18 34 E), is situated in northern Poland within the Complex of Chełmno and Vistula Landscape Parks at 91 m a.s.l. The climate is classified as warm temperate, fully humid with warm summers (Kottek et al., 2006) or cold without dry season with warm summer (Beck et al., 2018). Average annual precipitation in this region is between 500-550 mm and average annual air temperature is between 7.5-8.0 • C. The peatland is dominated by Sphagnum fallax, Eriophorum vaginatum, Oxycoccus palustris, Andromeda polifolia, Aulacomnium palustre, and Drosera rotundifolia (Boiński & Boińska, 2004). The experimental site included also shrubs and young trees such as Betula nana and Pinus sylvestris, respectively.
To simulate warming, we used Open Top Chambers (OTCs), which are commonly used in manipulative experiments in situ (e.g., Delarue et al., 2011;Jassey et al., 2013a;Marion et al., 1997), while water table depth was manipulated by adding or removing peat (Lamentowicz et al., 2016;Reczuga et al., 2018). The advantage of manipulative field experiments is that they are performed under realistic environmental conditions with community composition and abiotic drivers as they appear and work in the field (Underwood, 2009). Field experiments were approved by The Regional Directorate for Environmental Protection in Bydgoszcz (WPN.6205.70.2011.KLD). The experimental design with plots and treatments are given in Fig. 1.
In August 2012, experimental plots were defined according to a full factorial design involving two temperatures and three water table depths. The temperature increase effect was manipulated using OTCs or let under ambient temperature as control (AMB). OTCs are passive warming systems that allow increasing mean temperature by ca. 1.2 • C to 1.8 • C (Marion et al., 1997). The hexagonal OTC chambers were constructed with transparent polycarbonate material. The internal diameter between opposite corners was 250 cm at the base. To allow for air circulation, the OTCs were placed 10 cm above the soil surface. We manipulated water table depth by adding or removing 10 cm layers of peat in 1-m 2 plots. For each plot four subplots (50 × 50 cm and 30 cm thick) were cut. They were attributed to different measures (e.g., moss sampling for this study, respiration, biomass). Each plot belonged to one of three water table treatments: control (subplots cut and put back in place, abbreviation: CON), wet (10 cm of peat removed beneath each subplot before putting the subplot back in place, abbr.: WET), dry (10 cm of peat added from the wet treatment before putting the subplot back in place, abbr.: DRY). CON treatment was cut and put back in place to control for the disturbance introduced by cutting. Each plot was a combination of one of the three water table treatments and one of the two warming treatments. All six combinations were replicated three times, giving a total of 18 plots (subplots within the experimental plot belonged to the same treatment). Treatments were assigned to the plots randomly. Air temperature was recorded in each plot at 30 cm height using HOBO U23 Pro v2 data loggers (Onset Computer Corporation, USA) and the water table depth (WTD) was measured at each sampling (given in cm below the soil surface). Whenever we are referring to the measured values we use abbreviation WTD, while term ''water table treatments'' is used when we refer to the levels of manipulation (i.e., DRY, CON, and WET). A subset of the data from the experiment described in this study has already been published elsewhere (Jassey et al., 2018;Lamentowicz et al., 2016;Samson et al., 2018). The experimental design was described by Lamentowicz et al. (2016), where further details can be found. The effect of warming manipulation on temperature has been published in Samson et al. (2018), a study describing influence of warming and water table treatments on carbon dioxide release.

DNA extraction, PCR amplification and next-generation sequencing
Two to three individual Sphagnum stems (top three cm, including capitula) were sampled in three different seasons in each of the plots on May 16th (spring), August 20th (summer) and November 7th (autumn) in year 2013 and fixed in LifeGuard TM Soil Preservation Solution (MoBio, Carlsbad, CA USA). The plots were placed in monospecific Sphagnum fallax lawns and therefore we did not consider the species level identification of the sampled Sphagnum. In total 54 samples were taken (6 combinations of treatments * 3 replicates * 3 seasons). We sampled only the top part of the mosses as previous studies proved this part to be the most sensitive to the changes in the water table depth and warming manipulations (Basińska et al., 2020;Reczuga et al., 2018). DNA was extracted using the PowerSoil R DNA isolation kit (MoBio, Carlsbad, CA USA) according to the manufacturer's instruction. The DNA was extracted from two to three sampled Sphagnum mosses, which is approximately 0.3 -0.5 g of material per plot. PCR amplification of the SSU rDNA V9 region was carried out with eukaryotic-specific primers 1380F (CCCTGCCHTTTGTACACAC) and 1510R (CCTTCYGCAGGTTCACCTAC) (Amaral-Zettler et al., 2009). PCR reactions were conducted according to the following conditions: denaturation at 95 • C for 3 min, 25 cycles at 94 • C for 30 s, 57 • C for 30 s and 72 • C for 60 s and final extension at 72 • C for 10 min (Amaral-Zettler et al., 2009). PCR reactions were run with a SensoQuest Labcycler (GmbH, Göttingen, Germany) with 3 l of environmental DNA extract, 4 µL of 5X Colorless GoTaq R Buffer, 0.6 µl of each primer, 0.6 µl of dNTP Mix 10 mM (Promega, Dübendorf, Switzerland) and 0.2 µl of 0.05 U/ µl Go Taq Polymerase (Promega, Dübendorf, Switzerland). Each PCR reaction was performed with a positive and a negative control. Negative controls included PCR reaction mix with DNA extract replaced with water. The purification step was done using the Wizard R SV Gel and PCR Clean-Up System (Promega, Madison, WI USA). Library preparation and paired end sequencing was performed at the iGE3 Genomics Platform of the University of Geneva, Geneva, Switzerland using Illumina Hiseq technology (2 × 150 bp).

Sequence analysis
The computational pipeline used to analyse the reads includes the following steps: trimming of the tagged primer sequences, quality check, removal of rare sequences (i.e., OTU's occurring less than 3 times in the full dataset), clustering, and taxonomic assignation. For a given read, the quality check was based on moving windows of 50 nucleotides. The probability of incorrect base call was calculated for every nucleotide based on the phred score and arithmetic mean of these probabilities was calculated for every window. To avoid artefactual sequences; for the same purpose, we kept only reads that were present at least three times in the full dataset (De Vargas et al., 2015). Sequence clustering was then performed using Swarm v.  (Pearson, 1999). The sequences assigned to Metazoa and Embryophyceae were excluded from further analysis. In order to remove possible false positive sequences only OTU's occurring at least 10 times in the dataset were retained for further numerical analyses. Based on the taxonomic assignation, each OTU was assigned to a functional group (autotrophs, mixotrophs, parasites, osmotrophs and phagotrophs) according to Table 1. The assignation of OTUs to the functional groups was based on the expert curation (Enrique Lara). OTUs annotated in PR 2 database with an unknown taxonomic identity (Guillou et al., 2013), were crosschecked individually by aligning them against the NCBI's nucleotide database using BLAST algorithm with default parameters.

Growing degree day
To link the micro-eukaryotic communities with warming, we used a growing-degree day (GDD) approach, also known as accumulated degree day (ADD). The GDD is widely being used to predict plant and insect phenology and has more recently been used to relate e.g., grasshopper and butterfly community changes to climate change (e.g., Cayton et al., 2015;Nufio et al., 2010).
where, T max are daily maximum air temperature in • C, T min are daily minimum air temperature in • C, T base is a base temperature, equal to 10 • C. For each sample, the GDD was calculated for 135 days-the number of days since the beginning of the year until the first sampling.

Numerical analysis
All statistical analyses were performed in R version 3.5.1 (R Core Team, 2012) using RStudio Version 1.1.423 (RStudio Team, 2012). Whenever measured water table depth is used as a variable, we call it WTD, while whenever term ''water table treatments'' is used we refer to the levels of manipulation (i.e., DRY, CON, WET). The warming treatment effect on GDD and water table treatment on WTD was tested using ANOVA followed by Tukey multiple comparisons of means. We tested for treatment effects (both warming and water table manipulation) on the diversity patterns of micro-eukaryotic communities using the Shannon diversity index, rarefied OTU richness and evenness. OTU richness was estimated using rarefy function in the vegan package (Oksanen et al., 2014) at the sample size of 2410 (minimum number of reads across all samples) to compensate for the variability of the sample sizes. The sequencing effort between the samples was compared by drawing rarefaction curves using rarecurve function and by comparing slope calculated using rareslope function of the vegan R package (Oksanen et al., 2014). The slope was also calculated at the sample size of 2410. To test the significance of differences along measured WTD and temperature gradient (calculated GDD) linear mixed effects models with measured WTD and calculated GDD as fixed factors and season nested in plot as a random effect to account for the differences between plots across time. The assumptions of homoscedasticity and normality were previously tested. The tests were performed using lme function in the nlme package (Pinheiro et al., 2019). To further test the correlation between diversity and WTD and GDD, we calculated Pearson's correlation using cor.test function.
Subsequently, to test the response of micro-eukaryotes to the GDD, measured water table depth (WTD (cm)) and seasons, at the community level, we performed an RDA (Redundancy Analysis) based on Hellinger-transformed OTU counts. The RDA was done using rda function in the vegan package (Oksanen et al., 2014). Significance tests of each variable and axis in RDA models were tested using permutation tests (anova.cca function in the vegan package). To identify micro-eukaryotic indicators of climate change, we used Dufrene-Legendre indicator species analysis (Dufrêne & Legendre, 1997) and multipatt function in the indicspecies package (De Cáceres & Legendre, 2009). To manually verify taxonomic assignation against more wholesome database, the selected indicators' (with the highest indicator value) sequences were cross-checked by aligning them against the NCBI's nucleotide database using BLAST algorithm with default parameters.

Warming and water table manipulation effects on microclimatic conditions
Mean maximum daily temperature was about 1.1-1.2 • C higher in the OTC than in the ambient plots (Samson et al., 2018). The warming effect varied seasonally and over daytime, reaching a maximum effect of 4.1 • C on 5th of May 2013 and causing a slight cooling effect during winter and during the night (Lamentowicz et al., 2016). Mean daily air temperature was calculated on the basis of 10-minute averages. For each sampling, the temperature of the month prior to the sampling was calculated as the average of the mean daily air temperature. This mean was higher in the OTC than in ambient plots in spring and summer periods (by 0.54 • and 0.43 • , respectively). In each season WTD was higher (i.e., lower water table) in DRY as compared to the CON and WET. Mean WTD in DRY was 15 cm, 46 cm and 25 cm in spring, summer and autumn sampling, respectively, while in CON it was nine cm, 40 cm and 19 cm and in WET it was eight cm, 40 cm, 19 cm (Table S1, Fig. S1). Significant differences were observed between CON and DRY as well as between WET and DRY (Tukey, p < 0.05), while no significant difference was observed between WET and CON (Tukey, p = 0.6). GDD differed significantly (ANOVA, p <0.05) between AMB and OTC across seasons, with mean GDD of 76, 732 and 549 in AMB spring, summer and autumn periods, respectively, while OTC mean GDD was 101, 847 and 615 in spring, summer and autumn periods, respectively (Table S2). Significant differences between GDD in AMB and OTC were observed at each season (Tukey, p < 0.05). The environmental variables in experimental plots are provided in Data S1.

Micro-eukaryotic community structure
The Illumina sequencing generated 37,804,202 raw eukaryotic SSU V9 reads. Of these, the number dropped to 29,791,631 after quality check. These sequences were then clustered in 2,043 OTUs, reduced to 1,397 OTUs after removing sequences assigned to Metazoa or Embryophyceae. The abundance of each of the 2,043 OTUs in experimental plots is shown in Data S2, while the dominant sequence of each OTU is shown in Data S3. For ecological analysis, all assignations with similarity below 80% were excluded, leaving 1,226 OTUs. The majority of OTUs were assigned to the following five eukaryotic supergroups in decreasing order of taxonomic richness (i.e., 614, 214, 152, 99 and 83 OTUs): Opisthokonta, Alveolata, Archaeplastida, Rhizaria, respectively. A total of 369 OTUs (26.4% of the total number of OTUs) were assigned to taxa with a similarity above 97%. Among these, 250 were assigned to fungi and 119 to other taxa. Fungi OTUs reaching 97% of identity with the database constituted 40% of all fungi while only 16% of the other taxa reached the identity threshold illustrating the knowledge gap between fungi and protists.

Warming and water table manipulation effects on micro-eukaryotic diversity
The rarefaction curves (Fig. S2) clearly showed that the sequencing effort was not saturated at the sample level. However, when considering the whole dataset, the rarefaction curve indicated that the majority of micro-eukaryotic diversity was recovered. To compensate for the saturation variability among treatments, the OTU richness was calculated on a rarefied community in order to compare the effect of the different treatments. We did not observe significant differences in the slope of the rarefaction curves among water table or warming treatments (ANOVA, p = 0.6 and p = 0.9, for warming and water table treatments, respectively; Fig. S3). Linear mixed effect models revealed that Shannon diversity, evenness and rarefied OTU richness differed significantly along WTD and GDD (ANOVA, p < 0.01, Table S3). All diversity indices declined significantly with increasing WTD (Fig. 2, cor = −0.3 for all diversity measures, p < 0.05). No significant correlation was observed between GDD and biodiversity metrics. Shannon diversity and OTU richness were higher in autumn as compared to summer and spring. No significant difference was observed between warming treatments. The Shannon diversity, evenness, OTU richness and rarefied OTU richness in each analysed sample are given in the Table S4.

Micro-eukaryotic community response to the experimental manipulation
The redundancy analysis (RDA) revealed significant correlations between micro-eukaryotic communities and WTD (anova.cca permutation test, p = 0.001), GDD (p = 0.001) and season (p = 0.001). The full RDA model explained 22.5%, most of this (16.6%) being explained by seasons. To disentangle the seasonal effects from the influence of other environmental factors, we performed RDA with season as a conditional variable (Fig. 3). Here again, WTD (p = 0.014) and GDD (p = 0.017) were significant. The partial RDA model explained 5.9% (p = 0.003) of the variance. RDA model with water level and temperature treatments as variables and with season as a conditional variable revealed significant differences between water level treatments (p = 0.001), while the difference between temperature treatments was insignificant (p = 0.147; Fig. S4).
Among the 1,226 OTUs, 216 were considered autotrophs, 52 mixotrophs, 42 parasites, 579 osmotrophs and 319 phagotrophs (Table 1). Eighteen OTUs that could not be placed phylogenetically within any phylum, and therefore could not be functionally assigned, were excluded from the analysis. In the DRY treatment in spring, we observed a higher relative abundance of autotrophs and phagotrophs and a lower relative abundance of osmotrophs and parasites as compared to the WET and CON treatments. No such difference between treatments was observed in summer and autumn (Fig. 4).

Micro-eukaryotic indicators of global change
The indicator species analysis with each treatment as a separate group, allowed identifying 109 indicator OTUs (Table S5). A total of 96 OTUs were DRY indicators, 10 were WET indicators and three were identified as CON indicators (p < 0.05). Among the 96 DRY indicators, 28 were assigned to Fungi, 23 to Chlorophyta, 17 to Ciliophora, 14 to Cercozoa, six to Dinophyta, two to Cryptophyta and Stramenopiles, one to Apicomplexa, Discoba, Mesomycetozoa and Streptophyta. The DRY indicator with the highest indicator value was OTU_X77 (100% similarity with Cortinarius sp.) which had an indicator value of 0.963. The relative abundance of this OTU was highest in autumn (Fig. 5). Among the 10 DRY indicators with the highest indicator value, five were assigned to Archaeplastida (including four assigned to Trebouxiophyceae), four to Fungi and one to Alveolata (Colpodidae; Table 2). The increase of the relative abundance of autotrophs in spring corresponded to indicator algae adapted to dry soil environment and capable of symbiosis with lichens, such as Elliptochloris, (Trebouxiophyceae, Metz et al., 2019). The relative abundance of OTUs assigned to Elliptochloris, predominantly terrestrial taxa (Gustavs et al., 2017;Rindi, Hodkinson & Jones, 2011), increased from 1% in CON plots in May to 6% in DRY plots in May (Fig. S5), showing a shift towards a more terrestrial community.
A total of 27 indicators were identified for ambient vs OTC, nine of which were indicators of ambient temperature and 18 were indicators of warming (p < 0.05; Table S6).

DISCUSSION
Micro-eukaryotes, as key components of terrestrial ecosystems functioning, are vulnerable to ongoing climate change, which threatens global biodiversity (Geisen, Wall & Putten, 2019;Urban, 2015) making it urgent to gain insight into upcoming changes. Microeukaryotes are vulnerable to extinctions (Cotterill et al., 2013) and species loss may lead to cascading effects (Pearse & Altermatt, 2013) and disrupt ecosystem functioning (Santschi et al., 2017). It is expected that in stable habitats where the majority of species are near their thermal optima, taxonomic diversity will decrease with warming (Woodward, Perkins & Brown, 2010). Analogically, in stable peatlands, where the majority of micro-eukaryotes are near their humidity optimum, the diversity in the Sphagnum layer can be expected to decrease under drier conditions. Here, we confirm these hypotheses as diversity was negatively correlated with WTD. The diversity decrease might result in local loss of specialized species adapted to permanently water-logged conditions. These disappearing species may be replaced by taxa better adapted to new conditions. Conserving biodiversity is viewed as essential in part because our current knowledge does not allow to state which species are critical to the functioning of ecosystems and provide resilience and resistance to global changes (Chapin III et al., 2000). This is particularly true for micro-eukaryotes, whose significance in functioning of ecosystems has only recently been re-brought to light and which we know have important and sometimes unrecognized functions (Geisen et al., 2017).
The community composition of Sphagnum-associated micro-eukaryotes has only recently started being studied through molecular approaches. High throughput   sequencing (HTS) studies revealed that taxa previously believed to appear almost only in aquatic environments are present in moss-associated communities. For example, Dinoflagellates were recently reported in moss-associated communities (Heger et al., 2018) and Chrysophyceae and Kinetoplastida in soils (Lentendu et al., 2018). We also recorded these three groups in our study. As we gain insight into the community composition of micro-eukaryotes, the information on the function of the micro-eukaryotes associated with Sphagnum remains largely unknown. Identifying which micro-eukaryotes form close associations with Sphagnum mosses and what influence they have on their host and on the functioning of the ecosystem, remain open questions. Accordingly, the DRY plots were characterized by the presence of predominantly terrestrial taxa, among which many Trebouxiophyceae, such as Elliptochloris (Gustavs et al., 2017;Rindi, Hodkinson & Jones, 2011). Soil microalgae are better adapted to dehydration, rapid changes in temperature and intense solar radiation than their freshwater counterparts (Gray, Lewis & Cardon, 2007). Several members of the Trebouxiophyceae form symbiotic associations with lichenizing fungi (Metz et al., 2019). These associations are primarily terrestrial and most of them cannot survive permanently water-logged conditions (Hawksworth, 2000).
One of the indicators of drought (OTU_X77) is related to Cortinarius sp., (Agaricomycetes). This ectomycorrhizal fungi, commonly found in peatlands, is associated with the roots of Picea, Larix, Salix, and Betula (Thormann, 2006). Betula nana occurred in our plots and Pinus sylvestris grew in proximity of the plots, and both of these species could thus be the host for the OTU_X77. Encroachment of shrub and tree species is observed in pristine and drained peatlands in response to water loss and/or warming (Berg et al., 2009;Fay & Lavoie, 2009). It determines a shift in plant formation towards forest ecosystem. This transition increases water losses through evapotranspiration (Fay & Lavoie, 2009). Our observation of the drought indicator OTU_X77 may, therefore, be an early sign of these transition. However, contrary to our expectation, we did not observe an overall increase in diversity and relative abundance of fungi.
The HTS approach allows for DNA-based species identification and biodiversity assessment (Taberlet et al., 2012) but does not directly inform on the species' function, activity or metabolic state. While functions can, to some extent, be inferred from taxonomy (Adl et al., 2019), detailed knowledge about the function of many protists is still missing. Nevertheless, our study allows already to identify taxa which should be studied in more detail in priority to better understand how the observed changes in their abundance will affect ecosystem functioning.
The presence of these new taxa suggests a shift in the species composition and structure of microbial communities in response to water table drawdown towards terrestrial taxa. We also observed an increase in the diversity and relative abundance of terrestrial algae during the late spring, at the time of spring blooms (Fig. 4). Earlier algae blooms can be triggered by climate warming (Peeters et al., 2007) as warming might physiologically facilitate algal growth (Barton et al., 2003). Shifts in algal blooms timing are known to affect biological interactions within food-webs, such as competition (Peeters et al., 2007). Therefore, further studies are necessary to better understand by which mechanism drought stimulates the appearance of terrestrial algae and its consequences for the food-web. The drought simulated in this work, as a result of the manipulation, was probably more severe than the simple water table fall of about 10 cm. Possible cause of such scenario is a change in the peat position in boundary layer, and so altered evapotranspiration leading to more extreme drying. We can also expect more convective effects further enhancing the drought effect.
Changing biodiversity is affecting ecosystem functioning and the resilience of ecosystems to environmental change (Chapin III et al., 2000). For example, increased species richness may accelerate the decomposition of peat as a result of synergistic effects (Salonius, 1981). These effects are likely to be observed in species-poor ecosystems, where the occurrence of new species entails new functionalities (Vitousek & Hooper, 1994). In species-rich ecosystems, the impact of increased species richness on ecosystem processes is likely to be lowered due to functional redundancy (Chapin III et al., 2000;Johnson et al., 1996). Although there is no universal link between species diversity and ecosystem processes, certain processes are being fulfilled only by a handful of species and loss of these species might have huge consequences for ecosystem functioning (Chapin III et al., 2000;Kardol et al., 2016). Due to the scarcity of invertebrates in Sphagnum, micro-eukaryotic communities play major roles in the functioning of these ecosystems. Identifying Sphagnum-associated species which are vulnerable to climate change and inferring their function is useful to better predict future changes in the underlying peatland functioning and possible species loss (Midgley et al., 2002).
In a changing climate, the vulnerability of ecosystems is more likely to depend on community composition than on biodiversity (Chapin III et al., 2000). Changes in the relative abundance in favour of autotrophs at the expense of osmotrophs might affect the functioning of the ecosystem either by decreasing or by increasing decomposition rates, depending on how the food web structure responds. Increases in decomposition rates are, however, likely to occur deeper in the soil horizon were most of the decomposition processes take place, while our study investigated only the top part of the moss stem, where living Sphagnum dominates. In the DRY treatment, we identified some fungal indicators and we can expect that the appearance of these taxa might entail new functionalities in the ecosystem. Indeed, in the same experiment, (Jassey et al., 2018) did observe an increase in multifunctionality of enzymes in the DRY treatment. As pointed out by Kostka et al. (2016) Sphagnum-associated microbes might act as keystone species regulating C and N flow in peatlands. Changes in their community may therefore have consequences for the overall functioning of peatlands and their feedback on climate change.

CONCLUSIONS
Our study revealed substantial changes in the diversity and community structure of micro-eukaryotes, both at the OTU and functional levels, in response to experimental manipulation of temperature and water table depth, confirming our first hypotheses. Regarding the responses to water table variation, we observed a decrease in abundance and diversity of micro-eukaryotes, an increase in the relative abundance and a decrease in the diversity of eukaryotic micro-algae along with the water table depth. The increase in the number of autotrophs was due to the occurrence of predominantly terrestrial taxa (e.g., Elliptochloris, Trebouxiophyceae), indicating a shift from ''Sphagnum community'' to a ''terrestrial community''. Furthermore, we showed a decrease in the relative abundance of osmotrophs, including Fungi and parasites, including Oomycota (Peronosporomycetes). Overall, our work provides insight into the composition of Sphagnum-associated microeukaryotic communities and their response to drought and warming. We also show the potential of these organisms as indicators of ongoing changes. Identifying indicators of climate change using HTS might be a useful tool to identify state of the ecosystem and the direction of changes.