Trophic position, elemental ratios and nitrogen transfer in a planktonic host-parasite-consumer food chain including a fungal parasite.

Parasitism is arguably the most commonly occurring consumer strategy. However, only a few food web studies assess how well stable isotopes reflect the trophic position of parasitic consumers and results are variable. Even fewer studies have measured the nutrient transfer by parasitic consumers, hindering an assessment of their role in nutrient transfer through food webs. Here we used a food chain consisting of a diatom as host, a chytrid as its parasitic consumer and a rotifer as the predatory consumer of the chytrid, to assess the trophic position of all three food-chain components using their natural 13C and 15N isotope signatures, and to measure the nitrogen transfer from the host via the chytrid to the rotifer by tracing 15N of a labelled host up the food chain. Additionally, we measured the carbon to nitrogen (C:N) ratios of all food-chain components. Natural isotope abundance results showed no clear 15N enrichment in the chytrid or rotifer relative to the primary producer. However, estimates of nitrogen transfer indicated that about 14% of host nitrogen was transferred per day from host to chytrid during infection epidemics and that some of this nitrogen was also transferred onward to the rotifer. Moreover, C:N ratios decreased with trophic level, suggesting that the chytrid provided a high-quality food source to the rotifer. In conclusion, our results support the "mycoloop". The mycooloop proposes that chytrid infections allow the transfer of nutrients bound in large, inedible phytoplankton to zooplankton through the production of edible transmission spores, thereby rerouting nutrients back into the food web.

Introduction

Food webs describe the transfer of energy and nutrients through ecosystems based on trophic interactions. A substantial portion of consumers in food webs is parasitic consumers of free-living organisms (Dobson et al. 2008; class="Species">Kuris et al. 2008), but the occurrence and role of class="Chemical">parasitic consumers have been neglected in most food web studies, including aquatic ones (Lafferty et al. 2008). Even though class="Chemical">parasitic consumers dominate food web links (Lafferty et al. 2006), only few studies assess the troclass="Chemical">phic class="Chemical">position of class="Chemical">pan class="Disease">phytoplankton parasitic consumers and their role in nutrient transfer from host via parasitic consumer to zooplankton (Kagami et al. 2007). Chytrids, fungal parasitic consumers of phytoplankton, have been proposed to add previously unrecognized trophic links and to change the flow of carbon (C) in aquatic ecosystems (Grami et al. 2011; Kagami et al. 2014; Rasconi et al. 2014). Chytrids also play a role in regulating the dynamics and population densities of phytoplankton hosts and in the structure of pelagic plankton food webs (Ibelings et al. 2004). For instance, epidemics of parasitic chytrids on phytoplankton can increase host genetic diversity (Gsell et al. 2013), decrease uni-algal bloom size and duration, allowing competing species to thrive [see references in (Frenken et al. 2017a)] and thereby play a role in the seasonal succession of phytoplankton (Van Donk and Ringelberg 1983). Nevertheless, physical and chemical factors, together with grazing, have been considered to be the major controlling factor of phytoplankton populations, and most aquatic food web models still exclude parasitic consumers (Frenken et al. 2017a).

class="Chemical">Chytrid class="Chemical">pan class="Disease">infections of large phytoplankton have been suggested to be ecologically important for food web functioning. The “mycoloop” proposes that chytrid infections of phytoplankton transfer elements from large or inedible phytoplankton to zooplankton through the production of edible transmission propagules and thereby change the flow of nutrients through the food chain (Kagami et al. 2014). For example, large diatom species such as Synedra (25–400 μm) are inedible to common zooplankton species such as the rotifer Keratella, and the elements contained in the diatom cells were thought to be lost from the pelagic food web by sedimentation (Ibelings et al. 2004). However, chytrid fungi parasitizing these large diatoms take up nutrients from the host cells and produce free swimming zoospores, which in turn, can be eaten by zooplankton (Kagami et al. 2007), including rotifers such as Keratella (Frenken et al. 2018, 2020). In this way, chytrids directly link inedible phytoplankton to zooplankton (Kagami et al. 2014) (Fig. 1). Excretion of organic matter from phytoplankton cells may be taken up by bacteria which then can be consumed by small-bodied zooplankton, leading to an alternative pathway for nutrient transfer from inedible phytoplankton to zooplankton (Shniukova and Zolotareva 2015). This leakage of organic matter may increase with chytrid infection, possibly leading to higher bacteria numbers that could intensify this route (Senga et al. 2018). Thus, the mycoloop may be an important route establishing or enhancing the flow of nutrients in food webs that include inedible phytoplankton and parasitic consumers (Frenken et al. 2018; Haraldsson et al. 2018). To the best of our knowledge, the actual amount of nutrient transfer via the mycoloop has not yet been measured.

Fig. 1

Diagram of the mycoloop. The food web system includes the inedible diatom (Synedra), the obligate parasitic consumer of the diatom (chytrid) with a sessile (sporangium) and a motile (zoospore) life stage, and the rotifer (Keratella), which can consume the chytrid zoospores but not the host diatom. While Synedra is inedible to Keratella, its nutrients may still be transferred to the rotifer via infection propagules (zoospores)

Diagram of the mycoloop. The food web system includes the inedible diatom (class="Species">Synedra), the obligate class="Chemical">parasitic consumer of the diatom (class="Chemical">pan class="Chemical">chytrid) with a sessile (sporangium) and a motile (zoospore) life stage, and the rotifer (Keratella), which can consume the chytrid zoospores but not the host diatom. While Synedra is inedible to Keratella, its nutrients may still be transferred to the rotifer via infection propagules (zoospores)

The presence of class="Chemical">chytrids may not only affect the quantity of food that is transferred from the inedible class="Chemical">phytoclass="Chemical">plankton to zooclass="Chemical">plankton, but also its quality in terms of nutritional value. Zoosclass="Chemical">pores of class="Chemical">pan class="Chemical">chytrids are assumed to provide a source of high-quality food to zooplankton as they are nutrient rich as shown by their relatively low carbon to nutrient ratio (Kagami et al. 2007; Frenken et al. 2017b), transfer host-derived essential lipids and synthesise sterols de novo (Gerphagnon et al. 2018). Yet, little is known about the ecological stoichiometry of the mycoloop, and only limited data is available about the actual amounts of carbon (C) or nitrogen (N) transferred from freshwater phytoplankton to chytrids (see Grami et al. 2011; Haraldsson et al. 2018; Rasconi et al. 2014 for carbon fluxes and Frenken et al. 2017a, b for a review).

Natural abundances of class="Chemical">13C and class="Chemical">pan class="Chemical">15N isotopes can be used to analyse food web structure and to estimate contribution of different food sources (Layman et al. 2012). Nitrogen isotopic ratios (δ15N) show a gradual enrichment with trophic transfer (Minagawa and Wada 1984) and can be used to estimate the trophic position of organisms (Phillips et al. 2014). Carbon isotopic ratios (δ13C), on the other hand, stay relatively constant with trophic transfer and, therefore, inform about the food source of the consumer (Rounick and Winterbourn 1986; Post 2002). Consumers normally show an enrichment of approximately 3.4 ‰ in 15N and of 1 ‰ in 13C compared to their resource (Tilley et al. 2013). However, trophic fractionation (i.e. isotopic difference between consumer and resource) has been shown to vary considerably in laboratory and field studies with particularly variable outcomes for herbivores (Vander Zanden and Rasmussen 2001). Part of this variability has been associated with species identity, type of tissue analysed and the quantity or quality of the resource (Brauns et al. 2018). Trophic fractionation between parasitic consumers and their host shows large variability, where parasitic consumer 13C or 15N may either become depleted, remain unaltered or become enriched relative to its host (see Sabadel et al. 2019 for a review), rendering the question of the trophic position of parasitic consumers based on isotopic signatures inconclusive. Additionally, stable isotopes can be used for labelling studies or “stable isotope probing” studies (SIP) (Fry 2006). By enriching organisms with known amounts of heavy isotopes, 13C and/or 15N, the transfer of this label can be traced along trophic interactions to quantify the flux of nutrients from one trophic level to the next (Fry 2006). Hence, stable isotope analysis offers opportunities for improving our understanding of the role of chytrids in transferring nutrients and its trophic position in freshwater food chains.

Here, we assessed the trophic position of class="Chemical">chytrids based on isotoclass="Chemical">pic signatures and the transfer of N using a troclass="Chemical">phic chain of the diatom host class="Chemical">pan class="Species">Synedra sp., its chytrid parasitic consumer Zygophlyctis planktonica, and the rotifer Keratella cochlearis. These three species form a linear food chain as the rotifer can consume the zoospores of the chytrid (Frenken et al. 2020) but not the relatively large diatom host. First, to test whether stable isotope signatures reflected the trophic positions of all food chain components, natural abundances of 15N and 13C were assessed in host, infected host, chytrid zoospores and in rotifers exposed to a diet of either uninfected Synedra (inedible) or infected Synedra (producing edible zoospores). Second, to assess N-transfer through the food chain, the same experimental set up was repeated using 15N-enriched host to trace the flow of 15N from host to chytrid zoospores (quantitatively) and from uninfected or infected diatom host cultures to rotifers (qualitatively). Concomitantly, we assessed the C:N elemental ratios of all food chain components to evaluate changes in their nutritional quality.

Materials and methods

Model system

The experiments were performed using cultures of class="Species">Synedra sp. (also referred to as Ulnaria sclass="Chemical">p. (class="Chemical">pan class="Disease">Williams 2011); strain HS-SYN2 isolated from Feldberger Haussee, Germany), its host-specific chytrid parasitic consumer (strain SVdW-SYN-CHY1 isolated from Melzer See, DE) and Keratella cochlearis (isolated from Lumen Pond, The Netherlands). The chytrid has been identified as Zygophlyctis planktonica (Seto et al. 2020).

class="Species">Synedra sp. is a single-celled, needle-shaclass="Chemical">ped class="Chemical">pennate diatom. The average cell length of our class="Chemical">pan class="Species">Synedra population was about 70 µm, which is larger than the reported preferred algal particle size of < 12 µm for the rotifer Keratella (Edmondson 1965), making Synedra cells likely too large to be easily ingested by Keratella (Frenken et al. 2016). Chytrid infection of the diatom host starts with free swimming zoospores (diameter ca 2–3 µm; Seto et al. 2020) finding and attaching to a host cell. Subsequently, the zoospores encyst and form epibiontic sporangia while penetrating and digesting the host through a rhizoidal system. Within the sporangium, the next generation of zoospores is formed and finally released through rupture of the sporangium (Doggett and Porter 1996). Each infection is fatal and prohibits further reproduction of the host (Canter et al. 1992). Zoospores are small enough to be consumed by the rotifer Keratella cochlearis and their relatively low carbon to nutrient ratios, essential fatty acid profiles and de novo synthesis of sterols make them a valuable food source to zooplankton (Frenken et al. 2017a, b; Kagami et al. 2014; Gerphagnon et al. 2018). The tested Keratella species has been shown before to prey on zoospores of chytrids, even surviving and reproducing on a zoospore diet if food quantity was sufficient (Frenken et al. 2017a, b, 2020).

All organisms were grown under laboratory conditions on artificial class="Chemical">WC medium (with addition of class="Chemical">pan class="Chemical">silicate, Guillard and Lorenzen 1972) at 18 °C and an incident light intensity of 60 µmol photons m−2 s−1 at a 16 h light: 8 h dark cycle in an incubator (MLR-350, Sanyo Electric Co., Ltd. Japan). Prior to the experiments, diatom and chytrid cultures were acclimatised to the experimental conditions in semi-continuous batch cultures for at least 2 weeks (about 10–12 generations). Diatom and chytrid cultures were grown in 1 L glass Erlenmeyers. Rotifers were cultured in 4 mL wells using 12-well plates (VWR collection, Radnor, USA) as they did not grow well in large glass Erlenmeyers and were fed ad libitum with the green alga Chlorella sorokiniana on WC medium under the same temperature and light conditions as the experiments. All cultures were monospecific but not axenic.

Experimental set-up

The same experiment was performed twice, first without, and subsequently with class="Chemical">15N labelling of the host class="Chemical">poclass="Chemical">pulation. The natural-abundances exclass="Chemical">periment assessed the troclass="Chemical">phic class="Chemical">position of the diatom host, class="Chemical">pan class="Chemical">chytrid and rotifer in a simple food chain based on their natural 15N and 13C isotope ratios. The N-transfer experiment quantified the transfer of nitrogen (N) from the host to the chytrid and assessed the qualitative transfer of N onwards to the rotifer. Both experiments were set up identically, except for labelling the Synedra culture used to start the N-transfer experiment with 10 atom% 15N nitrate (15N NaNO3, Sigma-Aldrich).

Each experiment consisted of three treatments (Figure ESM 1). Treatment 1 acted as control for class="Species">Synedra class="Chemical">poclass="Chemical">pulation growth and class="Chemical">poclass="Chemical">pulation growth dilution of class="Chemical">pan class="Chemical">15N labelling. Treatment 2 assessed rotifer population growth with Synedra as only food source and N-transfer when co-culturing Synedra and Keratella. Treatment 3 consisted of two consecutive steps, with 3a) quantifying infection dynamics and N-transfer from host to chytrids by exposing Synedra to chytrids, followed by 3b) co-culturing half of the infected Synedra cultures with Keratella to assess rotifer population growth with Synedra and chytrid zoospores as food source and N-transfer. The experiments were run in batch cultures and each treatment was replicated three times. Before starting the N-transfer experiment, the Synedra stock culture was 15N-labelled by growing it in 10 atom% 15N NaNO3 enriched WC medium for 16 h, followed by filtrating the culture over a 5 µm mesh size plankton net, resuspending it in unlabelled WC medium and starting the experiment within an hour.

The experiments were started with an average initial concentration of 650 cells mL−1 of class="Species">Synedra in all three treatments, which allows several generations of class="Chemical">poclass="Chemical">pulation growth before nutrients can become limiclass="Chemical">pan class="Chemical">ting. Treatments 1 and 3a were conducted in 1 L glass Erlenmeyer flasks. Exposure to chytrids in treatment 3a was realised by adding a chytrid zoospore suspension to achieve a starting concentration of 500 zoospores mL−1. The zoospore suspension was prepared by gravity filtration of a heavily infected Synedra culture through a 5 µm mesh size plankton net. This mesh size excludes Synedra (average cell length 70 µm) and let zoospores pass through as their average diameter is 2–3 µm (Seto et al. 2020). At day 8 of treatment 3a, half of the volume of these Synedra-chytrid cultures was harvested, set to 20% infection prevalence by adding uninfected Synedra cells (15N labelled for the N-transfer experiment) and used to start treatment 3b. Treatments 2 and 3b were conducted in 24-wells (i.e. 2 × 12-well) per replicate. Rotifers were collected by pipetting and washed five times in WC medium to remove any remaining Chlorella cells. Each well then received 25 rotifers and either 4 mL of uninfected Synedra culture (Treatment 2) or 4 mL of 20% infection prevalence Synedra-chytrid culture (Treatment 3b). As about 900 rotifers were needed to surpass the detection limit of the elemental and isotope analysis, 24 wells constituted one replicate.

During the experiments, Erlenmeyer flasks and plates were shaken daily and redistributed randomly in the incubator to ensure averaged light conditions. Treatment 1 was run for 4 days (~ four host generations), to allow assessment of exponential population growth of the host, Treatments 2 and 3b were run for 5 days each (~ one rotifer generation), to allow incorporation of nutrients derived from feeding on zoospores or bacteria into the body tissue, and Treatment 3a was run for 8 days (~ 8 class="Chemical">chytrid generations), to allow high class="Chemical">pan class="Disease">infection prevalence and, therefore, sufficient zoospore biomass build up for stable isotope analysis.

Sampling

Each replicate was sampled at start and end of the treatment. Start and end samples for treatments in glass Erlenmeyers were taken as subsamples from each replicate Erlenmeyer (Treatments 1 and 3a). To achieve sufficient biomass for stable isotope analysis, start samples for treatments in 12-well plates were taken as subsamples from the starclass="Chemical">ting cultures used to fill the three sets of 12-well class="Chemical">plates class="Chemical">per treatment, while end samclass="Chemical">ples were taken by class="Chemical">pooling 24 wells (i.e. 2 × 12-well class="Chemical">plates) class="Chemical">per reclass="Chemical">plicate (Treatments 2 and 3b). In treatment 3a, samclass="Chemical">ples of class="Chemical">pan class="Species">Synedra-chytrids cultures were also taken at days 4, 5 and 6 to monitor population growth. Synedra and Synedra-chytrid populations of treatments 1, 2 and 3a were sampled for uninfected and infected host population counts, zoospore counts, infection prevalence and particulate organic carbon (POC) and nitrogen (PON) of two size fractions (> 5 µm: hosts + hosts with attached infections; < 5 µm: zoospores). Rotifers were sampled at the end of treatments 2 and 3b by counting the rotifer population per well, collecting and subsequently pooling rotifers of 24 wells for isotope analysis and elemental analysis. After removal of the rotifers, the Synedra and Synedra-chytrid cultures were also pooled by 24 wells and sampled for population counts, infection prevalence, POC and PON analysis. Population count samples were fixed with Lugol’s iodine solution (for diatoms, final concentration of 1% v/v) or with Glutaraldehyde (for zoospores, final concentration of 0.5% v/v) and stored at 4 °C in the dark until counting. To assess POC and PON of Synedra, Synedra-chytrid as well as pre-filtered zoospore suspensions, known volumes of each experimental unit were filtered at the start and end of the treatments over glass fiber filters (GF/F Whatman 1825-047, pore size ~ 0.7 µm). To determine the contribution of bacteria to POC and PON, we filtered the same amount of culture also over GF/C filters (Whatman 1822-024, pore size ~ 1.2 µm) assuming that most bacteria will not be retained on filters of this pore size. Rotifers were counted, collected by pipetting, washed in demi-water and transferred into a droplet of water in a tin capsule (standard size 8 × 5 mm) per replicate (i.e. 24 wells pooled). Filters and tin cups were dried at 60 °C and stored dry and dark until analysis.

Sample analysis

Population growth rates and infection prevalence

class="Chemical">Poclass="Chemical">pulation counts of class="Chemical">pan class="Species">Synedra, chytrid-infected Synedra and zoospores were performed using an inverted fluorescence microscope (DMI 4000B; Leica Microsystems CMS GmbH, Mannheim, Germany) following the Utermöhl method (Lund et al. 1958). Prior to counting, the chytrid-infected samples were stained with Calcofluor White (C40H44N12O10S2 Fluorescent Brightener 28; Sigma-Aldrich), which binds to the chitinaceous structures of chytrid sporangia and fluoresces under UV light (Rasconi et al. 2009). As zoospores did not react with the stain, we relied on visual detection in unstained samples. For each sample, at least 400 cells or 40 fields of view (FOV) were counted which allows a ± 10% accuracy (Lund et al. 1958). Rotifer populations per well were counted using a stereomicroscope (Leica WILD MZ8, Leica Microsystems B.V., Son, The Netherlands).

Elemental analysis and isotopic ratios

The class="Chemical">POC and class="Chemical">pan class="Chemical">PON samples were used to measure the elemental C and N composition as well as the δ13C and δ15N values in the different trophic levels of both, the natural abundances and the N-transfer experiment. The samples on filters were prepared for analysis according to standard methods (Teece and Fogel 2004). The samples were analysed using an elemental analyser (EA) (Flash 2000 Elemental Analyser, Thermo Scientific Bremen, Germany) coupled to an isotope-ratio mass spectrometer (Delta V Advantage Isotope Ratio Mass Spectrometer, Thermo Scientific Bremen, Germany) via a Conflo IV. Three internationally recognized standards [Arndt Schimmelmann Biogeochemical laboratories Indiana University; acetanilide, mean ± standard deviation (SD): δ13C = − 29.53 ± 0.01 ‰ and δ15N = 1.18 ± 0.02 ‰, used for calibration; urea (mean ± SD: δ13C = − 8.02 ± 0.05 ‰ and δ15N = 20.17 ± 0.06 ‰, used as standard and casein (Elemental Microanalysis Ltd; mean ± SD: δ13C = − 26.98 ± 0.13 ‰ and δ15N = 5.94 ± 0.08 ‰ used as standard] were repeatedly measured during the analysis to monitor instrument performance (i.e. 02 ‰ for 13C and 0.3 ‰ for 15N) and calculate the isotopic composition (13C and 15N) of the samples.

The isotope ratio δclass="Chemical">13C and δclass="Chemical">pan class="Chemical">15N of the samples were expressed as the relative difference in isotope ratio between the sample and international reference standard in parts per thousand: where δX is either δ 13C or δ 15N and R is the isotope ratio 13C/12C or 15N/14N in the sample and in the standard, respectively. The Rstandard to which the samples were compared to were Vienna PeeDee Belemnite (V-PDB; 0.0112372) for carbon and air-N2 (AIR-N2; 0.003663; (Merriam et al. 2002)) for nitrogen. A positive δX value indicates a higher proportion of the heavy isotopes in the sample relative to the respective standard (Hobson and Clark 1992).

Data analysis

Population growth rate and infection prevalence

The counts of class="Species">Synedra, class="Chemical">pan class="Disease">infection and rotifers were used to calculate their net population growth rate per replicate and treatment using the following equation: where X1 and X2 are the cell densities at the start and end of the treatment, respectively; and t2–t1 the duration of the treatment in days. To determine the prevalence of infection, Synedra cells carrying living infections (i) and uninfected Synedra cells (ui) were counted. The prevalence of infection (P) was then calculated according to Rasconi et al. (2009):

C:N ratio

The class="Chemical">carbon to class="Chemical">pan class="Chemical">nitrogen (C:N) ratio of uninfected Synedra, infected Synedra, zoospores and rotifers was calculated based on the C and N elemental composition of the samples. Comparison of the EA measurements obtained from GF/F and the GF/C filters allowed to assess the contribution of bacteria to the C:N ratio. The C:N ratio was expressed by atom, which was calculated by dividing the mass of C and N by their respective molar masses.

Trophic position and N-transfer

The trophic position of the class="Chemical">chytrid in resclass="Chemical">pect to its host class="Chemical">pan class="Species">Synedra and its predatory consumer Keratella was assessed using the δ13C and δ15N values obtained from the natural-abundances experiment. The N-transfer within our experimental food chain was quantitatively calculated for the transfer from Synedra to the chytrid and qualitatively assessed for the transfer from chytrids to rotifers using the δ15N values of the N-transfer experiment based on GF/C filters to reduce the isotope signal from bacteria as much as possible.

We expressed the N-transfer from class="Species">Synedra to zoosclass="Chemical">pores as the atom% class="Chemical">pan class="Chemical">15N excess (15Nxs) which is the increase of atom% 15N values in the zoospores relative to the atom% 15N values in the relevant source (i.e. Synedra population). The calculations are based on the equations described by Werner and Brand (2001) and Dugdale and Wilkerson (1986). By reformulating Eq. 1, Rsample was calculated as which was then used to calculate the atom% 15N as

and consequently, pan class="Chemical">15Nxs which is the atom% class="Chemical">pan class="Chemical">15N excess in the sample over the source as

The relevant atom% class="Chemical">15N source for the zoosclass="Chemical">pores harvested on day 8 is the atom% class="Chemical">pan class="Chemical">15N of uninfected Synedra cells they have been growing on. Given the chytrid generation time of about 26 h (unpublished data), we estimated the atom% 15N value of the Synedra cells of day 7 while taking into account the 15N label dilution in the host during exponential growth by fitting an exponential model to the 15R data of the host control (treatment 1) (Merriam et al. 2002) as where 15R1 and 15R2 are the isotopic ratio 15N/14N at start and end of treatment 1, respectively; and t2–t1 the duration of the treatment in days. Using the dilution 15R rate, we extrapolated the 15R value of the Synedra population on day 7 to calculate the atom% 15N source value for Eq. 6. The N-uptake rate of the zoospores was calculated assuming a relevant assimilation time of one chytrid generation.

Finally, we assessed the pan class="Chemical">15N uclass="Chemical">ptake rate by the class="Chemical">pan class="Chemical">chytrid on the sampling day as

considering the unclass="Disease">infected class="Chemical">part of the class="Chemical">pan class="Species">Synedra population on day 7 of treatment 3a as relevant N source to the zoospores. Hence, we multiplied the mean N content of uninfected Synedra cells (mean: 0.0034 g N cell−1; SD: 0.0001 g N) by the population density of uninfected Synedra (mean: 20,337 cells mL−1; SD: 5611 cells mL−1) present on day 7 in treatment 3a.

The class="Chemical">nitrogen transfer from the zoosclass="Chemical">pores to class="Chemical">pan class="Species">Keratella was qualitatively assessed by comparing the 15Nxs of rotifers in the N-transfer experiment to that of rotifers in the unlabelled controls (natural-abundances experiment) within their respective treatments (2 and 3b). While rotifers in treatment 2 were presumably starving due to the inedibility of Synedra, the rotifers in treatment 3b had food available in form of chytrid zoospores.

Statistical analysis

Data were tested for normality and equality of variance prior to analyses. Outliers in the EA-IRMS analysis were detected following the criteria by Rousseeuw and Hubert (2011), resulclass="Chemical">ting in the removal of five out of 114 δclass="Chemical">pan class="Chemical">15N values (Table ESM 2). All confidence intervals are at 95% level. 95% confidence intervals were run to determine differences in the same treatments between experiments and between comparable treatments within experiments. We compared for differences in population growth rates of the same treatments between experiments to assess whether 15N labelling had an influence on the growth rates; and between treatments within experiments to test for treatment effects. Specifically, we compared population growth rates of Synedra with and without exposure to rotifers (treatments 1 vs. 2) as well as the infection rate and zoospore production with and without exposure to rotifers (treatments 3a vs. 3b). Significant differences in population growth of rotifers exposed and non-exposed to infection were assessed with a t test. We also run t tests to determine significant difference in atom% 15N of rotifers fed with uninfected or infected Synedra (treatments 2 and 3b). Changes in C:N ratio with increasing trophic level were tested with a linear regression by numerically coding trophic levels (Post 2002) as host = 1; host-chytrid mixed cultures = 1.5; chytrids = 2, rotifers = 3. Qualitative differences in 15Nxs of rotifers exposed to infected and uninfected Synedra cultures were assessed with T tests analyses. Statistical analysis and graphing were performed in R (R-Core-Team 2012) using RStudio (RStudioTeam 2015).

Results

Population growth rate

While the main focus of our study was on stable isotope results, we assessed population growth rates of unclass="Disease">infected and class="Chemical">pan class="Disease">infected Synedra, chytrids and rotifers exposed to either uninfected or infected Synedra cultures to evaluate whether the overall performance of populations was similar between comparable treatments or between experiments. We expected high-population growth rates of uninfected Synedra alone and in co-culture with rotifers and much reduced or even negative population growth rates of infected Synedra due to mortality inflicted by chytrids. We also expected no population growth in rotifers exposed to uninfected Synedra and low but positive population growth in rotifers exposed to infected Synedra. The confidence interval results indicate that population growth rates per species per treatment showed some differences between experiments but responded overall similarly (Fig. 2). Population growth rate of uninfected Synedra in treatment 1 and 2 were clearly higher than Synedra growth rates in the infected treatments in both experiments (i.e. non-overlapping confidence intervals in natural-abundances and N-transfer experiment), with the highest population growth rate under labelling conditions. In treatment 2 of both experiments, the confidence intervals of population growth rates of Synedra exposed (glass Erlenmeyer) and non-exposed to rotifers (plastic plates) overlap, indicating a comparable population growth rate under both conditions. In treatment 3, the confidence intervals of population growth rates of infected Synedra (treatment 3a) and infected Synedra exposed to rotifers (treatment 3b) do not show much difference between the experiments. The confidence intervals of population growth rate of rotifers from treatment 2 (exposed to uninfected Synedra) and treatment 3b (exposed to infected Synedra) showed little difference between treatments or experiments; however, population growth rates of rotifers in treatment 2 were much less variable and closer to zero while the population growth rates of rotifers in treatment 3b showed wider spread and included higher values. Additionally, the t test results showed that in treatment 3, the population growth rate of rotifers was significantly higher than in treatment 2 (t(12) = 3.49, p = 0.0075). The growth rates of infection per treatment were similar in both experiments. The confidence intervals showed that population growth rates of infection (treatment 3a) are significantly higher compared to infection exposed to rotifers (treatment 3b, Fig. 2).

Fig. 2

Summary of population growth rates (95% confidence interval, N = 3) of different species and species combinations (Synedra, Synedra exposed to rotifers, infected Synedra, infected Synedra exposed to rotifers, rotifers, infection and infection exposed to rotifers) of the three treatments (T1, T2, T3a and T3b) and the two experiments (natural-abundances and N-transfer experiments). Treatments were performed in Erlenmeyer flasks or in 12-well plates (indicated with an asterisk)

Summary of population growth rates (95% confidence interval, N = 3) of different species and species combinations (class="Species">Synedra, class="Chemical">pan class="Species">Synedra exposed to rotifers, infected Synedra, infected Synedra exposed to rotifers, rotifers, infection and infection exposed to rotifers) of the three treatments (T1, T2, T3a and T3b) and the two experiments (natural-abundances and N-transfer experiments). Treatments were performed in Erlenmeyer flasks or in 12-well plates (indicated with an asterisk)

Trophic position

Natural-abundances experiment—trophic position based on δ15N and δ13C values

To test whether δclass="Chemical">15N and δclass="Chemical">pan class="Chemical">13C values reflect the predetermined trophic position of diatom host, chytrids and rotifers, we calculated the means and standard deviations of the δ15N and δ13C values per species using the values of the natural-abundance experiment (Fig. 3). Rotifers were enriched in δ13C relative to Synedra and chytrid zoospores, while zoospores showed no δ13C change relative to their host (Fig. 3). Moreover, rotifers showed no or even negative 15N fractionation relative to Synedra or the chytrids while zoospores had variable but on average 1.5 ‰ higher δ15N values than Synedra.

Fig. 3

Bivariate plot of means and standard deviations of δ13C vs. δ15N values from the different predetermined trophic levels: uninfected Synedra, infected Synedra, Synedra with zoospore suspension, zoospores and rotifers without (treatment 2) and with zoospores of chytrids as food source (treatment 3b)

Bivariate plot of means and standard deviations of δclass="Chemical">13C vs. δclass="Chemical">pan class="Chemical">15N values from the different predetermined trophic levels: uninfected Synedra, infected Synedra, Synedra with zoospore suspension, zoospores and rotifers without (treatment 2) and with zoospores of chytrids as food source (treatment 3b)

C:N ratio of trophic groups

The C:N ratio of pan class="Species">Synedra samclass="Chemical">ples showed a wider variation comclass="Chemical">pared to that of class="Chemical">parasitic consumers and rotifers (Fig. 4). Moreover, the C:N ratio decreased with increasing troclass="Chemical">phic level (F(2, 2) = 28.89, class="Chemical">p = 0.032, with an R2 of 0.91). Additionally, GF/F filter-based results (i.e. filters including bacteria) showed slightly but consistently lower C:N ratios than the GF/C filters (excluding most bacteria).

Fig. 4

C:N ratios of the predetermined trophic levels: Representation of ratio of molar carbon to nitrogen (C:N ratio) of the filters GF/F (including bacteria, pore size ~ 0.7 μm) and the filters GF/C (excluding bacteria, pore size ~ 1.2 μm) filter measurements of Synedra, infected Synedra, zoospores and rotifers

C:N ratios of the predetermined trophic levels: Representation of ratio of molar class="Chemical">carbon to class="Chemical">pan class="Chemical">nitrogen (C:N ratio) of the filters GF/F (including bacteria, pore size ~ 0.7 μm) and the filters GF/C (excluding bacteria, pore size ~ 1.2 μm) filter measurements of Synedra, infected Synedra, zoospores and rotifers

N-transfer

Quantitative N-transfer from Synedra to zoospores

The δclass="Chemical">15N values obtained from the N-transfer exclass="Chemical">periment were used to quantify the class="Chemical">pan class="Chemical">nitrogen transfer in our system. The N-uptake by zoospores on day 8 was expressed as 15Nxs of zoospores relative to Synedra, and showed an average of 0.098 (± 0.025; Table 1). The average N-transfer rate from Synedra to the zoospores was 191.6 (± 57.3) µg N L−1 h−1 given a standing stock of uninfected host containing 1.8 g N L−1 (Table 2). Hence, at day 7 of the experiment, when the prevalence of infection was 55%, about 14% of the N content of uninfected Synedra was transferred to the chytrids per day.

Table 1

Atom% 15N values of zoospores and host and 15Nxs of zoospores relative to the host show parasite enrichment

Atom% 15N zoospores	Extrapolated atom% 15N Synedra on day 7 based on growth dilution of label	15Nxs of zoospores relative to Synedra
0.629	0.555	0.074
0.653	0.555	0.098
0.688	0.555	0.133
0.626	0.555	0.070
0.648	0.555	0.093
0.678	0.555	0.123
	Average	0.098
	SD	0.025

An exponential loss model on the Synedra control (treatment1) (Eq. 7) was used to calculate the growth dilution of the 15N label to estimate the atom% 15N of the host for day 7. Uptake by zoospores on day 8 was expressed as 15Nxs of zoospores relative to the Synedra host. Average and standard deviation (SD) of 15Nxs of zoospores relative to their host was calculated for subsequent N-uptake rate estimation

Table 2

N-uptake rates (µg N L−1 h) of the parasite were calculated using the absolute uptake (µg N L−1) based on the GF/F and GF/C zoospore suspension filters of day 8 (Table 2)

Type filter	µg N L−1 zoospores	Uptake (μg N L−1)	Absolute N-uptake (µg N L−1)	Time (h)	N-uptake rate (μg N L−1 h-1)
GF/F	64,772.3	0.042	2708.83	26.4	181.27
GF/C	56,173.8	0.066	3690.47	26.4	208.01
GF/F	57,354.0	0.101	5777.97	26.4	288.51
GF/C	42,039.8	0.038	1605.19	26.4	111.86
GF/F	51,199.8	0.061	3108.14	26.4	179.91
GF/C	38,729.8	0.091	3508.16	26.4	179.92
				Average	191.58
				SD	57.27

Average and standard deviations (SD) N-uptake rates by zoospores was then calculated based on the period of one generation time of the parasite

Atom% class="Chemical">15N values of zoosclass="Chemical">pores and host and class="Chemical">pan class="Chemical">15Nxs of zoospores relative to the host show parasite enrichment

An exponential loss model on the class="Species">Synedra control (treatment1) (Eq. 7) was used to calculate the growth dilution of the class="Chemical">pan class="Chemical">15N label to estimate the atom% 15N of the host for day 7. Uptake by zoospores on day 8 was expressed as 15Nxs of zoospores relative to the Synedra host. Average and standard deviation (SD) of 15Nxs of zoospores relative to their host was calculated for subsequent N-uptake rate estimation

Qualitative N-transfer from zoospores to rotifers

The class="Chemical">nitrogen transfer from the zoosclass="Chemical">pores to the rotifers was assessed qualitatively by comclass="Chemical">paring the atom% class="Chemical">pan class="Chemical">15N of rotifers in the N-transfer experiment relative to that of rotifers in the unlabelled controls (natural-abundances experiment) within their respective treatments (not exposed to chytrids: treatment 2, exposed to chytrids: treatment 3b). The difference in δ15N values in the N-transfer experiment samples was significant for treatment 2 (mean = 137.9; SD = 16.2) and treatment 3b (mean = 332.5; SD = 11.5) with t (1.69) = − 14.699, p = 0.0087 (Table 3). This result suggests that rotifers took up some Synedra derived N in both treatments, but that they took up relatively more Synedra derived N in treatment 3b.

Table 3

Higher 15N enrichment in the rotifers with zoospores as food source: atom% 15N of rotifers in the N-transfer experiment relative to rotifers in the (unlabelled) natural-abundances experiment per treatment suggest that uptake of Synedra derived N took place in both treatments 2 and 3b but there was relatively more uptake in treatment 3b

Treatment	N-transfer experiment		Natural-abundances experiment
	δ15N	Atom% 15N	δ15N	Atom% 15N
2	126.422	0.411	0.815	0.365
2	149.312	0.419	2.343	0.366
2	NA	NA	1.590	0.366
3b	344.171	0.490	0.109	0.365
3b	321.089	0.482	0.837	0.365
3b	332.349	0.486	1.541	0.366

NA denotes not sufficient rotifer biomass for measurement

Higher class="Chemical">15N enrichment in the rotifers with zoosclass="Chemical">pores as food source: atom% class="Chemical">pan class="Chemical">15N of rotifers in the N-transfer experiment relative to rotifers in the (unlabelled) natural-abundances experiment per treatment suggest that uptake of Synedra derived N took place in both treatments 2 and 3b but there was relatively more uptake in treatment 3b

Discussion

To the best of our knowledge, this study is the first that examined the relative trophic position of a phytoplankton host, its class="Chemical">chytrid class="Chemical">parasitic consumer and a rotifer as class="Chemical">predatory consumer of the class="Chemical">pan class="Chemical">chytrid using their natural abundance stable of 15N and 13C isotopes and tracked the change in molar C:N ratios with trophic level. Additionally, we assessed the N-transfer from host to chytrids (quantitatively) and from chytrids to rotifers (qualitatively) using 15N-labelled host. Our results show no clear 15N enrichment in the chytrids or rotifers relative to the host, but a decreasing molar C:N ratio with increasing trophic level. Moreover, in our experimental conditions, chytrids took up about 14% of the host’s standing stock of N per day and passed N on to rotifers, showing that chytrids are well integrated in the food web.

Our results show that population growth rates were largely comparable within treatments and between experiments. The population growth rates of unclass="Disease">infected Synedra exclass="Chemical">posed and non-exclass="Chemical">posed to rotifers (treatments 1 and 2) were relatively similar, suggesclass="Chemical">pan class="Chemical">ting that Synedra growth is not affected by the presence of rotifers. Our results also show that there were only small differences in Synedra population growth rates between treatments performed in glass Erlenmeyer flasks (i.e. Synedra non-exposed to rotifers) or in plastic well plates (i.e. Synedra exposed to rotifers) and, therefore, we consider that Synedra growth rate is not affected by container type.

In the treatment 3, the class="Disease">infection strongly reduced the net class="Chemical">poclass="Chemical">pulation growth of class="Chemical">pan class="Species">Synedra overall. The net population growth rates of infection (based on prevalence of infection) as well as those of uninfected Synedra differed significantly between treatments 3a and 3b. In treatment 3a (no exposure to rotifers, performed in glass Erlenmeyers), prevalence of infection was higher, and the net population growth rate of uninfected Synedra was lower. These results align with previous studies performed by Van Donk and Ringelberg (1983), which showed that chytrid parasitism can drastically reduce a dominant diatom species population. Contrarily, in treatment 3b (exposure to rotifers, performed in plastic plates), the net population growth rate of uninfected Synedra was higher and the infection prevalence was lower. This result may indicate that the rotifers preyed on the zoospores and, therefore, fewer zoospores were available to infect Synedra. Rotifers have been shown to reduce chytrids zoospore density in another phytoplankton–host systems, although rotifer population growth showed to be limited by energetic needs and when zoospore density was insufficient, rotifer population decreased due to starvation (Frenken et al. 2017a, b, 2020).

The net population growth rate of class="Species">Keratella in treatment 2 was lower or negative comclass="Chemical">pared to the zoosclass="Chemical">pore-exclass="Chemical">posed rotifer class="Chemical">poclass="Chemical">pulation growth in treatment 3b, suggesclass="Chemical">pan class="Chemical">ting that Synedra is not a suitable food source and as a consequence rotifer’s mortality was higher than the reproduction rate. The net population growth rates of Keratella in treatment 3b (0.07–0.08 d−1) are largely in line with population growth rates of 0.07–0.1 d−1 reported in the literature for Keratella cochlearis feeding on good quality food sources at comparable temperatures (Walz 1983; Frenken et al. 2018). However, our experiment was shorter than the reproductive cycle of the rotifers (Frenken et al. 2020). Keratella exhibits a low population growth rate and limited offspring compared to other species of rotifers that can reach maximum growth rates of up to 0.8 d−1 at 18 °C (May and Bass 1998).

Trophic position based on natural δ13C and δ15N values

Natural abundance carbon isotopic composition

Estimates of δclass="Chemical">13C were variable, showing little difference in δ class="Chemical">pan class="Chemical">13C values between the chytrid and its host but a clear difference between rotifers and Synedra or chytrids. Doucett et al. (1999) proposed that parasitic consumers should be more enriched in 13C relative to their hosts, but the literature on host–parasitic consumer systems do not show a clear pattern of enrichment (see references in Sabadel et al. 2019). Rotifers showed an expected 1–2 ‰ enrichment in δ13C relative to Synedra and chytrid zoospores, aligning with the typical increase in δ13C per trophic level. Zoospores did not show a clear enrichment in δ13C relative to Synedra. The δ13C values were largely comparable between the different trophic levels, suggesting that rotifers, chytrids and Synedra were part of the same food web.

Natural abundance nitrogen isotopic composition

Results of δclass="Chemical">15N were variable, showing a slight increase in δclass="Chemical">pan class="Chemical">15N in zoospores relative to Synedra, but no or even negative δ15N for rotifers relative to either Synedra or chytrids. Although zoospores showed a 1.5 ‰ higher mean δ15N value relative to Synedra, variability between replicates was very high. Hence, it was not possible to distinguish trophic levels in our food web based on δ15N values of chytrids and rotifers. Doucett et al. (1999) argued that parasitic consumers that obtain all their nutrients from the host should show the same theoretical 3.4 ‰ enrichment in δ15N as predators feeding on prey. This number is based on a mean of variable measurements ranging from 1.3 to 5.3 ‰ (Minagawa and Wada 1984) and is related to the nitrogen compounds that are transferred from the host to the parasite. Therefore, if the parasite does not modify the structural composition of the nitrogen compounds, it will show an isotopic composition more comparable to its food source (Chikaraishi et al. 2007). However, variability in δ15N values across species can be rather high, even in very closely related species, which have been on the same diet (Macko et al. 1982; Hobson and Clark 1992). In some systems, parasites do show the expected 15N enrichment relative to their host (Doucett et al. 1999) but in other systems, the results of stable isotope analysis have been less clear or even contradictory. For instance, parasites in fish showed 15N depletion relative to their host (Deudero et al. 2002). Other studies (Deudero et al. 2002; Lafferty et al. 2008) showed that parasites can be depleted, enriched or have similar δ15N as compared to the host depending on the species of parasite and the host. In addition, the same parasite species in different hosts or different parasites species on the same host might have very different δ15N values (Lafferty et al. 2008). The reason for this inconsistency in the stable isotope response of parasites is still unresolved. Part of this variation in trophic discrimination factors of parasites may come from selective feeding on specific host substrates that differ in isotopic signature resulting in different enrichment patterns in the parasite (Deudero et al. 2002; Sabadel et al. 2019). In our host–parasite system, the chytrid infection kills the host and leaves an empty host cell without apparent residual cell contents. However, it remains unclear whether the chytrid actually consumes all cell contents of the diatom or whether there is leakage of specific compounds during the infection that could explain our result in a slight, but variable 15N enrichment in the parasite.

The rotifers also did not show enrichment in class="Chemical">15N relative to class="Chemical">pan class="Species">Synedra or the chytrid. Contrarily, they seemed to be depleted in 15N compared to the zoospores. The δ15N values obtained from the rotifers from treatment 2 (rotifers exposed to Synedra) were similar to those of uninfected Synedra. Low or even negative net population growth rates of rotifers in treatment 2 suggest that rotifers were starving. Moreover, pre-experiments showed that the population of Keratella exposed to Synedra as only food source collapsed and died within 9 days. This would agree with other studies that suggested that the size of Synedra cells is too large to be ingested by Keratella (Frenken et al. 2016). However, under starvation, an increase in δ15N would be expected (Gaye-Siessegger et al. 2007) which we do not observe in our results. Rotifers that were exposed to zoospores (treatment 3b) also showed 15N depletion compared to the δ15N values of Synedra and the zoospores, even though the population growth rate of rotifers in this treatment was comparable to growth rates under good food conditions (Frenken et al. 2018). It is also unlikely that the rotifer δ15N values are a legacy of the culture maintenance conditions as the food source (Chlorella sorokiniana) showed a higher δ15N (mean = 3.611; SD = 0.425, data not shown). However, we cannot fully exclude that the low δ15N of rotifers might reflect a change in their internal use of N due to starvation. How rotifers adjust their physiology when they undergo starvation conditions is not well understood (Kirk 1997). The protein content of rotifers can be very changeable and it is strongly related to their diet and cultivation conditions (Makridis and Olsen 1999). In other rotifer species, biomass, nitrogen and amino acid content decrease exponentially with time when they experience deprivation of food quantity or quality, especially at high temperatures (20–28 °C) (Makridis and Olsen 1999). These internal changes could explain why the rotifers did not show enrichment in δ15N compared to their food source.

Carbon to nitrogen ratio

In line with expectations, pan class="Species">Synedra showed the highest and most variable C:N ratio, while zoosclass="Chemical">pores and rotifers disclass="Chemical">played a narrower range with lower C:N ratios. Elemental comclass="Chemical">position of C, N and class="Chemical">pan class="Chemical">P differ between consumers and primary producers and these stoichiometric differences can be used as indicators of ecological processes such as nutrient cycling and trophic structure (Frost and Elser 2002).

Grazers typically have higher nutritional demands with lower and less flexible C-to-nutrient ratios than primary producers (Sterner and Elser 2002). Our results support these findings, where the class="Chemical">nitrogen content relative to class="Chemical">pan class="Chemical">carbon of zoospores and rotifers is significantly higher (i.e. lower C:N ratio) compared to that in Synedra. Consequently, chytrids may stoichiometrically upgrade the food for rotifers, which in turn may do so for higher trophic levels. We expected that the C:N ratio would decrease with higher trophic position as carbon is used in heterotrophic metabolisms while at the same time nutrients are becoming concentrated in higher trophic levels (Sterner et al. 1998; Boersma et al. 2008). We note that Synedra is relatively N rich in comparison to the Redfield C:N ratio of 6.6, suggesting that the diatoms were not N limited during the experiment. Also, the chytrid is relatively N-rich in comparison to literature values for pathotroph fungi (Zhang and Elser 2017) or aquatic saprophytic fungi (Danger et al. 2016).

The zoospore elemental composition seemed closer to that of rotifers while the class="Disease">infected Synedra values were more similar to unclass="Chemical">pan class="Disease">infected Synedra. Herbivorous consumers generally have higher nutrient demands than their plant food source and this higher requirement is reflected in their lower C:P and C:N ratios (Van de Waal et al. 2010; Hessen et al. 2013). Paseka and Grunberg (2019) showed that parasite C:N ratios can differ depending on life-cycle stage with lower C:N ratios during active reproduction. In line with earlier work (Frenken et al. 2017b, 2018), our findings show that zoospores appear to be efficient in transferring nutrients from their host to rotifers. This process can work in two ways: first by direct transfer of Synedra biomass to rotifers and upgrading the quality of the food, e.g. lower C:N ratios, for the rotifers. Second, the presence of chytrids might be linked to higher amounts of bacteria (personal observation), potentially through leakage of organic matter from the infected host. If we compare the GF/F filters (including bacteria) and the GF/C (excluding most bacteria), filters with more bacteria seem to show a lower C:N ratio, suggesting that the bacteria may also improve the quality of the food.

N-transfer based on 15N labelling experiment

Based on tracing the class="Chemical">15N label from host to the class="Chemical">pan class="Chemical">chytrid, we showed that ∼14% of the N content of Synedra was transferred to the parasitic consumers per day when the prevalence of infection was 55%. Although there are to date no studies that quantify the transfer of nutrients from phytoplankton to chytrids, Grami et al. (2011) developed a model to predict changes in carbon transport in a natural lake community due to chytrid parasitism on phytoplankton. According to this model, around 22% of the carbon of the phytoplankton is transferred to chytrid sporangia, 18% to the zoospores and 12.5% to zooplankton, resulting in less sedimentation loss of phytoplankton carbon and longer carbon path lengths. Our N-flux estimates suggest a comparable percentage of N transferred from hosts to zoospores and supports the hypothesis that chytrid parasitism can affect nutrient flows in aquatic food webs.

We assessed qualitatively the transfer of N from zoospores to rotifers as expressed in class="Chemical">15Nxs. Rotifers exclass="Chemical">posed to class="Chemical">pan class="Disease">infected Synedra showed higher atom% 15N compared to rotifers exposed to Synedra only, indicating an overall larger flux of N from resource to the rotifers when zoospores were available as food source. However, the rotifers experiencing starvation (Synedra only treatment) still showed a low amount of 15N labelling, suggesting that the rotifers were obtaining some 15N either directly from excreted extracellular material of Synedra or from bacteria feeding on these Synedra exudates. Rotifers exposed to chytrid-infected Synedra culture showed relatively more labelling compared to the Synedra only treatment, suggesting that these rotifers were obtaining more diatom host-derived nutrients. The mechanism for this is presumably through the direct intake of labelled zoospores as infected Synedra cells did not become more edible for the rotifer as the host silica frustules remain intact during and after infection. However, increased organic matter, including nitrogen, recycling through heterotrophic bacteria as a result of the parasitic infection (Senga et al. 2018) and, therefore, indirect labelling of the rotifers cannot be entirely excluded. Nevertheless, the labelling signal of the rotifers was very low when compared to zoospores and Synedra and we cannot exclude that rotifers were starving also in presence of zoospores. Rotifers can ingest ~ 5–10 µL d−1 (Rothhaupt 1995) and the density of zoospores at the end of the experiment was ~ 20 zoospores µL−1. The density of zoospores might have been too low for the rotifers to thrive despite zoospores being a good food quality source (Gleason et al. 2008).

Conclusions

Our results of the natural-abundances experiment confirm current knowledge that class="Chemical">chytrids comclass="Chemical">pletely declass="Chemical">pend on their host as food source as their δclass="Chemical">pan class="Chemical">13C was indistinguishable from their host. However, the expected 15N enrichment relative to their host was absent. Hence, assessment of the trophic position of the chytrid based on measuring stable isotopes of whole tissue (“bulk”) samples remains inconclusive. The potential of using stable isotopes for assessing the food web position of rotifers remained unresolved. Despite clear 13C enrichment of 1 to 2 ‰ relative to the food source as expected, we observed no 15N enrichment relative to host and parasitic consumer. While we cannot exclude starvation despite the presence of edible zoospores, net population growth rate in the zoospore-exposed treatment seemed not to support a severe starvation scenario. Our C:N ratio results showed that zoospores are relatively N rich and have a relatively similar C:N ratio as rotifers, suggesting that they are a high-quality food source for zooplankton. We could also confirm substantial transfer of N from host to chytrids and show some evidence that the host N was also transferred via chytrid infections to zooplankton, supporting the mycoloop concept and suggesting a role for chytrids in rerouting N flows from inedible producers to predatory consumers.

Future assessments of the trophic position of parasites may profit from using more informative stable isotope methods such as the compound-specific isotope analysis of amino acids, which allows much higher accuracy in trophic position estimation (Chikaraishi et al. 2007; Steffan et al. 2013; Sabadel et al. 2016). Furthermore, linking information on elemental ratios of organisms to their stable isotope signatures may help to assess the parasite trophic position, and understand the underlying mechanism of elemental imbalances between hosts, parasitic consumers and predatory consumers of parasitic consumers.

Below is the link to the electronic supplementary material.

Supplementary file 1 (pan class="Chemical">PDF 115 kb)