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Central European Journal of Immunology
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2/2013
vol. 38
 
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Experimental immunology
Assessment of the potential genotoxic and proapoptotic impact of selected cyanotoxins on fish leukocytes

Anna Sierosławska
,
Anna Rymuszka

(Centr Eur J Immunol 2013; 38 (2): 190-195)
Online publish date: 2013/07/08
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Introduction

Cyanotoxins, which are mostly secondary metabolites of cyanobacteria, are responsible for a wide range of negative health effects in the intoxicated aquatic and terrestrial organisms [1, 2]. During decay of cyanobacterial water blooms, the content of the bloom-forming cells is released into the water and cyanobacterial-derived toxic compounds may reach high concentrations, posing a threat to the organisms using such contaminated water. Except for well-described negative outcomes of intoxication with cyanotoxins, such as hepatotoxicity or neurotoxicity [3], there is an increasing number of reports indicating also other possible effects of the toxins, of not fully understood mechanisms, such as immunotoxicity or genotoxicity [4-6]. Microcystins (MCs), the most frequently detected cyanotoxins, are transported through plasmatic membranes by the multispecific organic anion transporting polypeptide superfamily (rodent Oatps, human OATPs), mainly expressed on hepatocytes [7], which makes the liver the target for these toxins. The main mode of action of MCs inside the cell is inhibition of serine/threonine phosphatases 1 and 2A (PP1 and PP2A). In addition to such effects as hyperphosphorylation of the cytoskeleton, disorders of vital cellular processes and, in consequence, the hepatocyte disruption [8], MCs are also able to induce DNA damage in these cells [8-10]. Moreover, it has been found that MCs may exert genotoxic changes not only in the liver, but also in such cells as fibroblasts, kidney cells [11] or in human lymphocytes [12, 13].

The other potent toxin produced by cyanobacteria is cylindrospermopsin (CYN). Its main mechanism of the toxic activity is irreversible inhibition of protein synthesis at the stage of elongation [14]. There is also another way in which CYN affects the cells and this manner needs previous toxin transformation by P450 enzymes [14]. Similarly to MCs, the main target for CYN is the liver. The studies on CYN genotoxic potential revealed that the toxin is also responsible for DNA damage in hepatocytes [15]. Recently, the toxin-induced formation of DNA single-strand breaks, increase in the frequency of micronuclei and nuclear buds in human peripheral blood lymphocytes exposed to CYN were reported [16].

On the other hand, there is nearly no information on possible genotoxic properties of the another frequently detected cyanotoxin, anatoxin-a (Antx-a). That toxin is a small alkaloid of strong neurotoxic activity. Only one study was found in the literature, which assessed toxin genotoxicity with the use of the umuC assay, in which the induction and expression of the umuC – lacZ reporter gene in bacteria Salmonella typhimurium was examined [17].

Fish, due to their habitat, are especially subjected to intoxication with cyanotoxins. There are only a few studies on the potential genotoxicity of cyanobacterial products on these organisms. Available data indicate that cyanotoxins may induce changes in nuclei of kidney cells, erythrocytes or embryos of different fish species [18-20]. Moreover, disruption of some vital functions of immune cells of fish was reported [21]. To the authors’ knowledge, there are no data on genotoxic effects of cyanotoxins on common carp (Cyprinus carpio L.) blood leukocytes.

The aim of the present work was to study the potential cytotoxic/genotoxic impact of three cyanotoxins – MC-LR, the most toxic variant among all MCs, CYN and Antx-a on common carp leukocytes. The comet assay (single cell gel electrophoresis, SCGE) was chosen because of its sensitivity and possibility to detect a wide range of DNA damage, such as single/double-strand DNA breaks, alkali labile sites (apurinic/apyrimidinic sites), DNA cross-links and base/base-pair damage in the cells. Additionally, to elucidate if the potential positive effects in the comet assay came from the cyanotoxin-induced genotoxic damage or they were the effects of nuclear fragmentation being a part of apoptosis, the percentage of apoptotic/necrotic cells in the leukocyte cultures was estimated.

Material and methods

Cyanotoxins



The following cyanotoxins in pure form were used: MC-LR and CYN purchased from Alexis (Switzerland) and Antx-a as a fumarate salt obtained from Tocris Bioscience (USA).



Experimental setup



In the study, the principles of laboratory animal care and the national laws (Opinion and Approval of Local Committee of Ethics No. 3/2009) were followed. Five common carps of either sex and mean body weight of 320 ±35 γ were obtained from the local breeding farm. Blood of fish was sampled from vena caudalis with heparin at 50 IU/mL and diluted with a Dulbecco’s Phosphate Buffered Saline (DPBS, BI, Israel). Leukocytes were isolated by blood centrifugation on Gradisol G (1.119 g/ml, Aqua-Med, Poland). Obtained cells (containing about 80% of lymphocytes) at a concentration of 5 × 106 cell/ml were suspended in complete RPMI 1640 medium (BI, Israel) containing 5% of heat-inactivated autological serum and 1% of penicillin/streptomycin solution. The cell suspension was dispensed to the 24-well microtitre plates in the aliquots of 1 ml per well with an addition of the appropriate toxin (MC-LR, CYN or Antx-a) at 0.5 g/ml and incubated at 24°C, 0.5% CO2, in the dark. After 18 h, the cells were harvested for further research.



DNA damage detection



The alkaline version of the comet assay was performed with the use of the CometAssay kit (Trevigen) to detect DNA damage in the cells after their exposure to the cyanotoxins. The producer’s protocol was followed. Shortly, leukocytes at 1 × 105 cell/ml were combined with low melting point agarose (LMA) and placed onto the slides. For each toxin, two slides were prepared. After 30 min incubation at 4°C in the dark, the cells were lysed with Lysis Solution for 60 min at 4°C. Then, the slides were immersed in Alkaline Unwinding Solution (pH > 13) for 60 min. Electro­phoresis was carried out with chilled Alkaline Electr­o­phoresis Solution (200 mM NaOH, 1 mM EDTA, pH > 13) at 1 V/cm, 300 mA, for 30 min at 4°C in the dark. The slides were immersed twice in dH2O and for 5 min in 70% ethanol. After drying, the slides were stained with SYBR Green I dye and viewed with a Nikon Eclipse Ti inverted fluorescence microscope. The comet images were analyzed with CASP ver. 1.2.3b1 software to determine the percentage of DNA within the comet tail (at least 100 nuclei per treatment and per control).



Apoptosis/necrosis detection



After the end of the incubation period, the cells were washed in DPBS and adjusted to the concentration of 5 × × 106 cell/ml. Then, leukocytes were stained with annexin V conjugated to fluorescein (An V FITC) and propidium iodide (PI) with the use of the Annexin-V-FLUOS Staining kit (Roche Diagnostic, Germany) for 15 min, according to the producer’s protocol. Stained cells were analyzed with the fluorescence microscope. Approximately 100 cells for each toxin treatment were counted. The cells with green fluorescence (An V FITC positive) were treated as apoptotic, while the cells with red fluorescence (PI positive) or with red and green fluorescence (An V FITC and PI positive) were treated as necrotic. The results are presented as a percentage of apoptotic/necrotic cells in the cultures exposed to the toxins in relation to the control cells.



Statistical analysis



Statistical analyses were performed by nonparametric Mann-Whitney U test with Statistica 8.0 software from StatSoft Inc. (Tulsa, OK, USA). P values < 0.05 were considered as statistically significant.

Results

DNA damage



Percentage of DNA in the tail of the exposed cells was significantly higher (p < 0.05) comparing to the control cells in two cases (Fig. 1). The most substantial DNA damage was observed in the cells exposed to MC-LR (Fig. 2B). The cells treated with CYN were affected to a lesser extent, however still to a significant degree (Fig. 2C). On the contrary, no signs of increased DNA fragmentation were observed in the cells incubated in the presence of Antx-a, and generally the images taken from the control cell nuclei did not differ essentially from those of Antx-a treated cell (Fig. 2A and 2D).



Apoptosis/necrosis



According to the phosphatidylserine dislocation in the plasma membrane, a high number of apoptotic cells was found after cell treatment with MC-LR. In the other cell populations, i.e. the CYN-treated and the Antx-a-treated, apoptotic cells were not substantially more frequent than in the control population. Moreover, there were low rates of necrosis in all studied cell groups, estimated on the basis of the cell membrane integrity (Fig. 3).

Discussion

Leukocytes, the cells of the immune system, play a crucial role in sustaining organism homeostasis. Thus, it is important to recognize the possible factors influencing their viability and normal functioning. It is known that some toxic substances, except for their direct effects on the target organ/tissue, are also able to disrupt various immune reactions. In these cases, in a hazard assessment, also changed or reduced abilities to fight pathogenic microorganisms or malignant cells should be taken under consideration.

The present study was conducted to examine whether well-known cyanotoxins, hepatotoxins MC-LR and CYN, as well as neurotoxin Antx-a, are able to exert cytotoxic/genotoxic effects on carp leukocytes.

The most evident results were obtained after the cell treatment with MC-LR. Observed high amounts of DNA in the comet tails after electrophoresis of the lysed cells indicated the presence of numerous DNA breaks. As the main components of the cell population were lymphocytes, the observed effects refer mainly to that kind of fish leukocytes.

The toxin-induced nuclear damage was also reported in many hepatocyte-based experiments, even at much lower concentrations than used in the present study [22-24], as well as in non-hepatocytic mammalian cells [25]. Human lymphocytes were relatively widely studied in that regard [12, 13]. In general, it is believed that MC-LR is a potent reactive oxygen species (ROS) inducer [8, 26]. In consequence, oxidative DNA lesions may be expected. Indeed, formation of 8-oxo-7,8-dihydro-2’-deoxyguanosine (8-oxo-dG), one of the most abundant products of DNA oxidation, has been found in the cells exposed to MC-LR [9, 27]. Moreover, the toxin inhibits enzymes involved in the repair of DNA damage [28]. On the other hand, Zegura et al. [25] did not observe any substantial DNA strand break induction in the NCNC human B-lymphoblastoid cell line exposed to the toxin at concentrations up to 10 g/ml for 2-16 h. It indicates differences among different cells as the susceptibility of the cells from different tissues may vary and some cell lines may possess other susceptibility than primary cells.

There are not many data from studies on fish cells in this respect. Recently, Wu et al. [20] has found that a cyanobacterial extract containing MC-LR was able to induce DNA and chromosome damage detected by the micronucleus assay and the SCGE assay in carp erythrocytes and kidney cells after a few-day in vivo exposure. Proapoptotic and cytotoxic influence of MC-LR on carp leukocytes, manifested as the increase of LDH leakage, increased number of apoptotic and necrotic cells, changes in intracellular GSH levels and affected phagocytic activity, was also observed by Rymuszka [21].

When assessing genotoxic effects with the comet assay, we have to consider some demands. The low viability of the studied cell population, as well as the cells during S phase, may give false positive results [29]. In the present study, there were not many necrotic cells, but we saw a high rate of apoptotic cells. During apoptosis, caspase-dependent degradation of nuclear DNA occurs [30]. It gives an increased amount of DNA fragments of a specified length, while the comet assay does not provide exact information on the size of fragments in the comet tail. That is why the assay alone may not testify to direct genotoxicity of the studied agent [29]. The method of apoptotic cell identification used here is based on detection of translocations of phosphatidylserine from the inner layer of the cell membrane to the outer one, which is a hallmark of early stages of apoptosis [31]. Whereas major DNA fragmentation is generally a late event in apoptosis [32], and late apoptotic cells stain with both An V FITC and PI, we think that a high rate of DNA in comet tails after MC-LR treatment is at least partially a sign of direct genotoxic disruption.

On the contrary, in the CYN-treated cell population the number of apoptotic cells was low. Nevertheless, an increased amount of DNA strand breaks was observed, indicating genotoxic potency of the toxin. Most studies concerning the cytotoxic/genotoxic influence of CYN was conducted with liver cells or hepatoma cell lines as CYN is known to be a hepatotoxin. These studies confirmed that the toxin is able to induce genotoxic damage, such as DNA strand breaks, the increase in the micronuclei number, nuclear buds and nuclear bridges [15, 33-35]. Similar effects were also observed in other metabolically active cells, e.g. kidney or ileum cells [34, 36]. It has been also found that inhibition of P450 enzymes abolished the genotoxicity induced by that toxin, which proves that CYN metabolites are mainly responsible for DNA damage [15]. Recently, Zegura et al. [16] has described the genotoxic effects of CYN on human lymphocytes, in which increase in the amount of DNA strand breaks, the induction of micronuclei and nuclear buds was observed after cell exposure to the toxin at a concentration of 0.5 µg/ml and below. In the present study, a similar increase in DNA fragments in comet tails was observed. On the other hand, Liebel et al. [37] did not detect any DNA damage in hepatocytes from Prochilodus lineatus exposed to the toxin at concentrations up to

10 g/ml for 72 h. In that study, however, increased reactive oxygen/nitrogen species levels and lipid peroxidation were found. In tilapia (Oreochromis niloticus) acutely exposed in vivo on CYN, increase in NADPH oxidase activity, a biomarker of reactive oxygen species formation, as well as lipid peroxidation and protein oxidation were described. At the same time, neither significant DNA oxidation nor reduction in glutathione levels was detected [38]. Based on the available data it can be concluded that CYN may be responsible for the oxidative stress and its consequences, but their range is varied and depends on the cell type.

The least studied toxin on its potential genotoxic activity is Antx-a. It has been detected that the toxin at a concentration of 0.5-2 g/ml is able to induce the expression of the umuC gene, one of the SOS genes, in Salmonella typhimurium TA 1535 (pSK1002) [17]. Induction of the SOS genes is a way of bacterial responses to genotoxic damage. Further studies with the use of the Ames test with different bacterial strains did not confirm mutagenic potential of that toxin (unpublished data). There is no information on the Antx-a influence on genetic material of eukaryotic cells. In the present study we did not observe any DNA damage in the toxin-exposed fish cells. There was no increase in the apoptotic cell number, either, however in our previous studies, when longer exposure time was applied, the neurotoxin occurred to be able to activate caspases 3/7 in carp cells. Additionally, alterations in phosphatidylserine location in cell membranes were seen at a toxin concentration of

1 g/ml, indicating dose-dependent proapoptotic activity of Antx-a [39].

In conclusion, MC-LR occurred to be the most toxic agent among the studied toxins toward carp leukocytes, exerting a proapoptotic and/or genotoxic influence. Some increase in DNA fragmentation was also detected after the cells treatment with CYN, not connected with the cell death. No effects of Antx-a on the treated cell under used in this study conditions were observed.



The authors declare no conflict of interest.

The study was financially supported by the National Center for Science, Grant No. N N304 306940.

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