Abstract
To elucidate the changes in the proportions of microcystin (MC)-producing Microcystis, non-MC-producing Microcystis and Anabaena strains during cyanobacteria blooms, we compared their fitness under different initial biomass ratios. Culture experiments were carried out with three cyanobacterial strains: single-celled toxic Microcystis aeruginosa PCC7806 (Ma7806), single-celled nontoxic Microcystis wesenbergii FACHB-929 (Mw929) and filamentous Anabaena PCC7120 (An7120). Growth curves expressed as biovolume, Ma7806 microcystin-LR (MC-LR) content (detected with HPLC and ELISA), and the culture medium dissolved total nitrogen and dissolved total phosphorous (DTP) were measured to monitor nutrient uptake. Results suggest that the dominant strain in competition experiments between Ma7806 and An7120 was mainly controlled by the initial biomass ratio of the two strains, but there was also evidence for allelopathic interactions, where MC-LR produced by Ma7806 played an important role in the competition process. However, Mw929 was always less competitive when co-cultured with An7120 regardless of initial biomass ratio. Culture medium DTP showed significant differences between competition experiments in all sets, suggesting that Mw929 could be more suited to low phosphorus environments than Ma7806 and An7120. Overall, the competitive ability of Ma7806 was stronger than Mw929 when co-cultured with An7120 in the case of excess nutrients and the results could well unravel the seasonal succession process of cyanobacteria blooms.
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Introduction
The increasing input of nutrients, mainly nitrogen (N) and phosphorus (P), to water is leading to increased eutrophication in many regions across the globe (Cloern 2001). The most obvious effect of eutrophication is its alteration of the food web, resulting in high levels of phytoplankton biomass that can lead to algal blooms (Anderson et al. 2002; Smayda 2004). Occurrences of cyanobacteria blooms around the world have increased in recent decades, and under favorable conditions Microcystis is the most important cyanobacterial genus responsible for water blooms (Hudnell and Dortch 2008; Azevedo et al. 2002). Most known species of Microcystis, such as Microcystis flos-aquae, M. aeruginosa, M. ichthyoblabe, and M. viridis, have been reported to produce a family of nearly 80 hepatotoxic peptides called microcystins (MCs) (Briand et al. 2009). MCs are responsible for liver failure in wild animals, livestock and aquatic life, and are a health hazard for humans through the use of water for drinking and recreation (Hoeger et al. 2007). The release of chemicals and toxins by plants, that affect their potential competitors for resources, is known as allelopathy (Lampert and Sommer 2007). Previous studies have found that allelopathic compounds produced by phytoplankton are active in succession events (Jüttner and Wu 2000; Vardi et al. 2002). Also, allelopathic compounds produced by submerged macrophytes might affect the succession of phytoplankton (Gross et al. 2003, 2007). Tillmann (2003) and Granéli and Hansen (2006) have pointed out that allelopathy and toxin production are enhanced by stress factors, such as unbalanced N and P ratios at limiting concentrations. To understand toxin variations and allelopathy in natural blooms, most early investigations were focused on toxic cyanobacterial species in the laboratory. However, other nontoxic species of Microcystis, for example M. wesenbergii (Xu et al. 2008), which also plays an important role in cyanobacterial blooms succession, has received less attention despite being distributed widely around the world including Asia (Son et al. 2005), Europe (Jasprica et al. 2005), America (Oberholster et al. 2006), and Oceania (Wood et al. 2005).
Filamentous cyanobacterial blooms (i.e., Anabaena blooms) have been observed to occur simultaneously with, or alternatively to, Microcystis blooms (Aktan et al. 2009; Solis et al. 2009; Vesna et al. 2010). Furthermore, in hypertrophic lakes or reservoirs, water temperature and other abiotic factors interact to allow high phytoplankton production (Robarts and Zohary 1992). Therefore, we conducted competition experiments between two Microcystis strains and Anabaena PCC7120 (An7120) in order to unravel the seasonal succession process indirectly during cyanobacteria blooms. These results will be beneficial not only for water agencies but also for future prediction of algal blooms.
Materials and methods
Cyanobacterial strains Microcycstis aeruginosa PCC 7806 (Ma7806) and Anabaena PCC 7120 (An7120) were originally obtained from the Pasteur Culture Collection of Cyanobacteria, France, and were kindly provided by the Freshwater Algae Culture Collection of the Chinese Academy of Sciences (FACHB-Collection). The nontoxic strain Microcystis wesenbergii FACHB-929 (Mw929) was isolated from Lake Dianchi in China and was also obtained from the FACHB-Collection. Mean cell dimensions of the three strains were measured using an ocular micrometer at ×400 magnification (Hill and Knight 1987). Cell densities of cultures were converted to biovolume (μm3 L−1) for each strain using the formula for the geometric shape roughly appropriate for the taxon (Hillebrand et al. 1999). In laboratory cultures, Ma7806 and Mw929 are single-celled and An7120 is filamentous (Table 1).
The three strains were axenic and inoculated in BG11 liquid medium, under a 12L/12D cycle with a light intensity of 30 μmol photons m−2 s−1 provided by cool white fluorescent tubes at 25 ± 1°C. Experiments were carried out in 500-mL conical flasks containing 300 mL BG11 liquid medium. All samples were run in triplicate and all flat-bottomed bottles were shaken by hand three times per day during the maintenance and experimental stages. Subsamples were taken at predetermined intervals from day 1 during the incubation period to determine cell numbers, examine dissolved total phosphorous (DTP) and dissolved total nitrogen (DTN) and extract MCs.
The initial biomass of each culture was determined from the concentration of chlorophyll a, then the cell number was counted and converted to biovolume. Two co-cultures were prepared: Ma7806 and An7120; Mw929 and An7120 (Table 2). Each sample was run in triplicate and was divided into subsamples for cell counting, for determination of MC content and for determination of extracellular DTN and DTP contents in the medium.
Measurement of cell number and biovolume
After staining with 1% acidified Lugol’s iodine solution, the cyanobacterial cells were counted under a microscope using a haemocytometer. The cells of An7120 and Mw929 were separated by sonication before counting. Cell counts were ultimately converted to biovolume by multiplying cell count by the estimated volume per cell.
Examination of DTN and DTP
Subsamples (10 mL) from the cultures were taken at predetermined intervals. The samples were firstly placed in Ultrasonic cleaning device (KQ 5200E) for 5 min, which promoted cells sinking to the bottom of the tube, as both Microcystis and Anabaena are known for the gas vesicles to assist buoyancy. Then they were centrifuged at 10,000 rpm for 12 min, and the supernatant was used to determine DTP and DTN after persulfate oxidation to nitrate (D’Elia et al. 1977) and orthophosphate, respectively. The nitrate was determined with a Szechrome NB reagent (Wynne and Rhee 1986), and the orthophosphate was determined by the phosphomolybdate method.
Microcystin extraction and analysis
Extraction of intracellular microcystin-LR (MC-LR) followed the method developed by Harada et al. (1988). Lyophilized cells were firstly sonicated and extracted three times with 5% (v/v) acetic acid. The extract was centrifuged at 8,000 rpm for 10 min and the supernatant was then transferred to a C18 cartridge (Sep-Pak; Waters Association). The C18 cartridge was activated with 10 mL methanol and 20 mL Millipore water and then impurities were eluted with 20% and 30% methanol separately prior to eluting MC-LR with 75% methanol. Finally, the eluted solutions were evaporated to dryness in a rotary vacuum evaporator, and then re-dissolved with 1 mL 50% methanol and stored at −20°C for high-performance liquid chromatograph (HPLC) analysis. Standard MC-LR was received as a gift from Dr. Wei Chen, IHB, CAS (>95% purity) (Chen et al. 2009) and MC-LR samples were analyzed by a Shimadzu CLASS-LC10 HPLC with a reverse C18 column (4.6 and 250 mm) in a run with 60% solution A (100% methanol) and 40% solution B (0.05% aqueous trifluoroacetic acid) over 20 min and diode array detector at 238 nm. The results showed that retention time of the MC-LR was 13.5 min.
Extracellular microcystin concentrations would be possibly below the detection limit of the high-performance liquid chromatograph (2 ng L−1). Therefore, they were determined using an enzyme-linked immunosorbent assay, which was performed according to the protocol of the microcystin plate kit (EnviroLogix, Inc.; Catalog no. EP022). This method is sensitive for low levels of microcystin (Pyo et al. 2005; Carmichael and An 1999). The assays were run in 96-well plates containing 0.1 mU enzyme (recombinant protein phosphatase 1A, catalytic subunit, Roche Applied Science), 1.05 mg para-nitrophenyl phosphate (Sigma) and 10 μL of sample or microcystin-LR (Sigma Biochemical). Water samples (5 mL per sample) were taken and stored at −20°C. In order to avoid false-negative or false-positive effects, we firstly transferred the supernatant to a C18 cartridge (Sep-Pak; Waters), eluting impurities. And then the diluted MC-LR extracted from water samples of 100 μL were added to test tubes pre-coated with polyclonal antibodies followed by addition of an enzyme-linked substrate. The antibodies were specific to MC-LR at low concentrations. Activity of the bound peroxidase was assayed as rate of hydrolysis of TMB (3,30,5,5,-tetramethylbenzidene), stopped with 1N HCl, and measured spectrophotometrically at 450 nm (absorbance peak) and 650 nm (turbidity blank) over 1 h. In the results, all reported toxin concentrations are microcystin-LR equivalents. And the detection limit was between 0.1 and 5 μg L−1.
In the results, all reported toxin concentrations are microcystin-LR equivalents. Unknowns, standards, and controls were all run in duplicate.
Statistics
Data are presented as mean±SD (standard deviation). All statistical analyses were computed with one-way analysis of variance (ANOVA) statistics using SPSS (Version 16.0), except for DTP in medium, which was analyzed with the t test for Mw929 co-culturing with An7120.
Results
Monocultures
All three strains flourished throughout the monoculture experiments, although their specific growth rates changed with time (Fig. 1). The growth rates of Ma7806, An7120, and Mw929 were 0.184, 0.285, and 0.117 day−1, respectively, in the exponential phase. Changes in MC-LR content showed a similar tendency to those of Ma7806 growth and reached a maximum in the mid exponential growth phase, but decreased in the late exponential growth phase (Fig. 1).
Changes in culture medium DTN and DTP were also estimated (Fig. 2). No significant differences in DTN concentrations were observed among the three strains (ANOVA, p > 0.05). However, a significant difference in DTP between Mw929 and An7120 was observed (ANOVA, p = 0.046 < 0.05).
Co-cultures of Ma7806 and An7120
The dominant strain under competition mainly depends on the initial inoculation biomass, that is, when Ma7806 dominated at the beginning, it continued to dominate until the end (Fig. 3a) and similarly with An7120 (Fig. 3c). However, when the initial inoculation amount of Ma7806 and An7120 was almost equal, both strains achieved similar growth rates (0.107 and 0.113 day−1) for the first 15 days, at which point An7120 started to grow faster than Ma7806 (Fig. 3b). However, both strains converged to similar biovolume densities by the end of the experiment (28 days). The maximum biovolume of An7120 in set (a) was much larger than that during the monoculture experiments while the growth of An7120 was seriously suppressed in set (c).
For MC-LR, the microcystin contents (fg cell−1) in sets (a) and (b) were much higher than that in set (c) (Fig. 4). The microcystin contents showed significant differences between sets (a) and (c) (ANOVA, p < 0.05) and between sets (b) and (c) (ANOVA, p < 0.01). Additionally, in set (b), the microcystin contents were positively correlated with the Ma7806 cell density, but were negatively correlated in set (c). Moreover, the extracellular fraction of MC-LR in the medium varied between different growth stages and growth conditions (Fig. 5).
No significant differences in culture medium DTN or DTP (p > 0.05; F = 0.173; df 1 = 2; and df 2 = 33) were found throughout the competition experiments between Ma7806 and An7120 in sets (a–c) (Fig. 6).
Co-cultures of Mw929 and An7120
An7120 biovolume eventually exceeded Mw929 biovolume for all three initial chlorophyll a ratios tested (Fig. 7). At the same time, the DTN (ANOVA, p > 0.05) showed almost the same trends (Fig. 8) for all three sets, while DTP showed significant differences between the three sets (t test, p < 0.05).
Discussion
In order to elucidate the changes in the proportions of MC-producing Microcystis, non-MC-producing Microcystis and Anabaena strains during cyanobacteria blooms, we compared their fitness under different initial biomass ratios. When Ma7806 and An7120 were cultured together, the dominant strain was largely determined by the initial biomass ratio between them. This result could further be attributed to the difference in growth rates between the two strains in the monoculture experiments, where the strains had no competitors. Oberhaus et al. (2007) carried out monoculture and competition experiments to compare the fitness of cyanobacterial strains Planktothrix rubescens and P. agardhii, cultured under various different conditions of temperature and light, and showed that there are significant differences in the growth rates of P. rubescens and P. agardhii in monoculture and competition experiments.
Moreover, the MC-LR concentration of Ma7806 was much higher in competition experiments than that inoculated in monoculture experiments; in particular, the concentrations of MC-LR in sets (a) and (b) were much higher than that in set (c), implying that the greater the competitive pressure the higher the cellular MC-LR content in competition experiments. This phenomenon results from two factors. The first can be assessed in terms of the costs and benefits of producing MC. MC is biosynthesized via a multi-enzyme complex requiring a high energy input, implying a high cost for the cell. Briand et al. (2008) suggested that, under cell growth-limiting conditions, the benefits of producing MC would outweigh the costs. In the monoculture experiment, Ma7806 had no competitor, so it did not invest resources in MC production. Meanwhile, Ma7806 did produce large amounts of MCs in order to outweigh other strains in competition experiments. The second factor is the possible allelopathic effect of Ma7806 on An7120 (Pflugmacher 2002; Schagerl et al. 2002; Sedmak and Elersek 2005), particularly when Ma7806 and An7120 were inoculated by similar amounts. In this case, their growth rates were initially similar (0.107 and 0.113 day−1, respectively), before An7120 became suddenly dominant from day 18 to day 27. Conversely, after day 27 the continually increasing MC-LR concentration suggests that the allelopathic effect was effective only if the intracellular content of MC-LR was sufficient to be released into the medium, when it would suppress the growth of An7120 (Pflugmacher 2002; Schagerl et al. 2002; Sedmak and Elersek 2005). In particular, MCs can function as inhibitors of photosynthetic activity (Hu et al. 2004; Sukenik et al. 2002). Therefore, to verify whether the allelopathic effect exists, the physiological experiments were analyzed (Fig. 9). The growth of An7120 was promoted or restrained when the concentration of MC-LR was below 0.1 μg L−1 or above 1 μg L−1, respectively. Therefore, the allelopathic effect occurred throughout the competition experiments. The maximum extracellular concentration of MC-LR was 0.0875 μg L−1 in set (a), while the maximum biomass of An7120 was much larger than that in the monoculture experiment. In set (c), the maximum extracellular concentration of MC-LR was 14.706 μg L−1 while the growth of An7120 was greatly suppressed by MC-LR, consistent with the physiological experiments. In natural water, the concentration of MC-LR varies dynamically and plays an important role in diversified algae biovolume construction. Moreover, the percentage of extracellular MC-LR in the medium ranged from 0.3% to 10.55% in set (a), from 13% to 23.47% in set (b) and from 0.244% to 63.7% in set (c), although Sedmak and Elersek (2005) reported that the extracellular fraction of MC-LR in the medium only accounts for approximately 1% the intracellular fraction, which might result from the different culture conditions. Above all, the results indicated that the more the biomass proportion of M. aeruginosa, the lager the concentration of MC-LR in medium. And hence, the quantity of MC-LR released into the natural waters varies during cyanobacteria blooms.
Additionally, neither DTN nor DTP showed significant differences in any experimental sets, which might result from the excess nutrients in the BG11 medium making competition between strains for nutrients unnecessary. Additionally, the initial total inoculated biomass was nearly identical in the competition experiments (Table 2), and total biovolume and cell size for each set were close so that the relative surface areas of the two strains were similar. This leads to similar rates of nutrient uptake, consistent with the monoculture experiments.
In the Mw929 and An7120 mixed culture experiments, Mw929 were eventually competitively suppressed by An7120 for all tested inoculation ratios. This result is mainly a function of two factors. The first is the subtle difference in growth rates between the two strains in the monoculture experiments, which inevitably affects their growth in the competition experiments. The second factor is cell size: Mw929 cells are much larger than An7120 cells. Mathematical theory predicts that the relative surface area of Mw929 will be much smaller than that of An7120; hence the latter will absorb nutrients more efficiently than the former. Furthermore, the decreases of nitrogen resources during the experiment will result in growth limitation of the cells (Fig. 7). However, under conditions of nitrogen deficiency, the nitrogen-fixing heterocysts will differentiate from vegetative cells in An7120 (Kaneko et al. 2001), and this characteristic will allow it to gain eventual dominance. Overall, Mw929 appeared to be weaker during competition with co-cultured An7120.
On the other hand, in Fig. 7, we could infer that the larger the proportion of Mw929 the greater the DTP in the medium when co-cultured with An7120, which indicates that Mw929 should be well accustomed to phosphorous deficiency conditions. Hence, the concentration of phosphorous could serve as a forecast of Mw929 blooms. Phosphorus often limits Microcystis growth in the natural aquatic environment. There are many reports of interactions between Microcystis and phosphorus. However, these reports focus mainly on the uptake of different forms of phosphorus by Microcystis (Yang et al. 2005) or its competitive utilization with other algae (Takeya et al. 2004) other than M. wesenbergii.
As we know, in most natural lakes in China, Microcystis blooms usually occur from early summer to late autumn. To a large extent, the phenomenon requires a suitable temperature. Microcystis have been found to have an optimal temperature for growth and photosynthesis at, or above, 25°C (Takamura et al. 1985; Robarts and Zohary 1987; Reynolds 2006; Jöhnk et al. 2008; Paerl and Huisman 2008). In natural waters, the temperature would be below 25°C from spring to early summer and hence Anabaena blooms could occur under favorable conditions; when the temperature reaches above 25°C, Microcystis species (i.e., M. aeruginosa and M. wesenbergii) would begin to grow rapidly and then Microcystis blooms would occur until late autumn; in late autumn, Anabaena blooms would occur again due to low temperature. During Microcystis blooms, the three strains always co-exist but their biomass proportion varies considerably at different periods. The biomass of M. aeruginosa is much larger than M. wesenbergii in the early period of Microcystis blooms, which our experiment results suggest is due to M. aeruginosa having a stronger competitive ability than M. wesenbergii under favorable conditions. Conversely, in the late period of Microcystis blooms, when the concentration of phosphorous in natural waters decreased markedly, the process of Microcystis blooms as well as that our experiment showed that M. wesenbergii was more tolerant to low phosphorus than M. aeruginosa. At the same time, the biomass of Anabaena varies considerably as well. According to our results, allelopathic effects of MC-LR on An7120 exist and the extracellular MC-LR concentration varies with different biomass proportion. When the temperature was below 25°C in spring, the biomass proportion of M. aeruginosa was usually smaller than Anabaena and the concentration of MC-LR released to natural waters would be much lower leading to promoting the growth of Anabaena. With increased temperature, the biomass proportion of M. aeruginosa would increase and the concentration of MC-LR in natural waters would also increase thus restraining the growth rate of Anabaena so that M. aeruginosa dominated for a long period. In the late period of Microcystis blooms, M. wesenbergii would dominate relatively for a short period until the temperature decreases to about 25°C and then Anabaena would dominate again. Overall, temperature, nutrients and microcystin jointly drive the succession of cyanobacteria blooms. Besides this, some other abiotic factors should be studied further.
In conclusion, our laboratory experiments demonstrate that the M. aeruginosa strain has a stronger competitive ability than M. wesenbergii under favorable conditions when co-cultured with An7120. The dominant strain in competition experiments between Ma7806 and An7120 mainly depends on the initial biomass ratio between the two strains. Differences in morphological forms and allelopathic effects of MC-LR produced by M. aeruginosa are considered to be the main factors controlling growth. Finally, we found that M. wesenbergii was tolerant to low phosphorus.
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Acknowledgments
The study was supported jointly by the National Natural Science Foundation of China (No.40971249), the National Basic Research and Development Plan (2008CB418002) and the National Programs of Water Body Pollution Control and Remediation (2008ZX07103-004-01, 2009ZX07104-005-3). We are also honestly grateful to Dr. Chen from IHB for providing of the MC-LR standard.
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Li, Y., Li, D. Competition between toxic Microcystis aeruginosa and nontoxic Microcystis wesenbergii with Anabaena PCC7120. J Appl Phycol 24, 69–78 (2012). https://doi.org/10.1007/s10811-010-9648-x
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DOI: https://doi.org/10.1007/s10811-010-9648-x