| Literature DB >> 29258177 |
Silvia Pichardo1, Ana M Cameán2, Angeles Jos3.
Abstract
Cylindrospermopsin (CYN) is a cyanobacterial toxin that is gaining importance, owing to its increasing expansion worldwide and the increased frequency of its blooms. CYN mainly targets the liver, but also involves other organs. Various mechanisms have been associated with its toxicity, such as protein synthesis inhibition, oxidative stress, etc. However, its toxic effects are not yet fully elucidated and additional data for hazard characterization purposes are required. In this regard, in vitro methods can play an important role, owing to their advantages in comparison to in vivo trials. The aim of this work was to compile and evaluate the in vitro data dealing with CYN available in the scientific literature, focusing on its toxicokinetics and its main toxicity mechanisms. This analysis would be useful to identify research needs and data gaps in order to complete knowledge about the toxicity profile of CYN. For example, it has been shown that research on various aspects, such as new emerging toxicity effects, the toxicity of analogs, or the potential interaction of CYN with other cyanotoxins, among others, is still very scarce. New in vitro studies are therefore welcome.Entities:
Keywords: cylindrospermopsin; cytotoxicity; genotoxicity; in vitro; oxidative stress
Mesh:
Substances:
Year: 2017 PMID: 29258177 PMCID: PMC5744122 DOI: 10.3390/toxins9120402
Source DB: PubMed Journal: Toxins (Basel) ISSN: 2072-6651 Impact factor: 4.546
In vitro cytotoxicity studies performed with Cylindrospermopsin (CYN).
| Toxin/Cyanobacteria | Experimental Model | Assays Performed | Exposure Conditions Concentration Ranges | Main Results | Reference |
|---|---|---|---|---|---|
| Purified extract from | Primary rats hepatocytes | Lactate dehydrogenase (LDH) activity | 0.5–5 µM for 0–18 h | After 18 h of incubation with 3.3 and 5 µM, significant cell death (40% and 67%, respectively) was found. No measurable cell lysis within the first 12 h of exposure to CYN, although slight signs of rounding were observed. | [ |
| Commercial CYN pure standard | Primary rat hepatocytes and KB cells | 3-(4,5-dimethylthiazol-2-yl)-2,5 diphenyltetrazolium bromide (MTT) assay | 0–10,000 ng/mL for 0, 24, 48, 72 h | Toxic effects were observed at after 72 h, being the LC50 40 ng/mL in the case of exposure to rat hepatocytes while in KB cells it was 200 ng/mL. | [ |
| Purified extract from | Primary rats hepatocytes | LDH release | CYN: 0.16–10 µM | When hepatocytes were exposed to 20 µM of RAC-CYN cell death increased from 14% to 23%, while in the case of CYN-DIOL cell death enhanced up to 38%. Similar results were observed in exposures to 10 µM CYN, 12.5 µM EPI-CYN and 50 µM EPI-DIOL with increases of 33.4%, 38.5% and 35%, respectively. | [ |
| Purified extract from | Primary rat hepatocytes; Caco-2 and HepG2 cells | MTT assay | 24 h to primary rat hepatocytes | None of the 7 isolates of | [ |
| Commercial CYN pure standard | Primary mouse hepatocytes | LDH release | 0.05–25 µM for 18, 21, 24 h | Time- and concentration- dependent increases in LDH leakage was observed after exposure to CYN. The EC50 at 18 h was 0.47 μM. The concentration response was very steep, with concentrations of 1 μM and above producing greater than 75% LDH leakage within 18 h whereas concentrations below 0.1 μM had no effect. | [ |
| Commercial CYN pure standard | HDF, HepG2, and Caco-2 cells | MTS assay and LDH leakage | 0.1–5 μg/mL CYN for 24, 48, 72 h | Although it was not possible to calculate the IC50 for the MTS assay due to lack of data for higher concentrations, a time-dependent effect was observed in all three cell types. However, no effect was observed in the LDH assay in rHepG2 and Caco-2 cells, but HDF cells reached 30% of the lysed controls at concentrations above 1 μg/mL CYN (2.4 μM) after 72 h. | [ |
| Purified extract from | CHO-K1 cells | Annexin V- fluorescein isothiocyanate/propidium ionide (FITC) apoptosis detection kit | 0.05–2 µg/mL for 3, 16, 21 h | CYN increases the frequency of necrotic cells in a dose and time-dependent manner, but very slight impact on apoptosis was observed. In addition, when cells are metabolic activated the susceptibility to necrotic cell death increases, whereas it has no impact on apoptosis. | [ |
| Purified extract containing CYN and deoxyCYN | HepG2, BE-2, Caco-2, MNA, HDF | Trypan blue exclusion test (TBET) and MTS assays | 0.1–5 µg/mL for 24, 48, 72 h | Both CYN and deoxyCYN exerted toxic effects to all exposed cells in a concentration and dependent way, being deoxyCYN slightly less cytotoxic than CYN. | [ |
| Commercial CYN pure standard | Primary human granulosa cells | MTT assay | 0–1 µg/mL for 2, 4, 6, 24, 48, 72 h | No effect was recorded in cells exposed up to 1 µg/mL in short 2–6 h exposures. However, cell viability decreased in a concentration-dependent way at longer exposures (24–72 h). | [ |
| Commercial CYN pure standard | C3A, HepG2, NCI-87, HCT-8, HuTu-80, Caco-2, and Vero cells | MTT assay and LDH leakage | 0.4–66 µM for 1, 2, 4, 6, 24 h | The 24 h IC50 for CYN cytotoxicity was set at 1.5 µM for hepatic cell lines (C3A and HepG2 cells), while for colonic cells (Caco-2) the IC50 was 6.5 µM. Similar onset was found in hepatic cells (C3A) in long-term exposures up to 7 days. No recovery of the toxicity caused by CYN was evidenced in C3A cells after exposure for 1–6 h. | [ |
| Commercial CYN pure standard | Vero-GFP cells | MTS (3-(4,5-dimethylthiazol-2-yl)-5-(3-carboxymethoxyphenyl)-2-(4-sulfophenyl)-2H-tetrazolium) assay | 0.1–100 µM for 4, 24 h | The IC50 found for CYN after 24 h was 5.9 µM. The use of other protein inhibitors indicated that the toxicity exerted by CYN was not only related to protein synthesis mechanism but other effects may contribute to the toxicity observed. | [ |
| Commercial CYN pure standard | CHO cells | Annexin V-FITC assay | 0.1–10 µM for 12, 18, 24, 48 h | CYN cause apoptosis at low concentrations (1–2 µM) and over short exposure periods (12 h). Necrosis was observed at higher concentrations (5–10 µM) and following longer exposure periods (24 or 48 h). | [ |
| Commercial CYN pure standard | PLHC-1 | Protein content (PC), neutral red uptake (NRU) and MTS assay | 0.3–40 µg/mL for 24, 48 h | Cytotoxic effects were observed in all the endpoints assayed in a time and concentration-dependent manner. Regarding the EC50 values, the most sensitive endpoint was PC for 24 h of exposure, with an EC50 of 8 µg/mL, and MTS assay for 48 h with an EC50 of 2.2 µg/mL. | [ |
| Purified extract containing CYN | Primary | NRU | 0.1–10 µg/L for 72 h | Cell viability decreased 8% in hepatocytes exposed to 0.1 and 1 µg/L. However, at the highest concentration assayed (10 µg/L) no significant change was observed in comparison to the control. | [ |
| Commercial CYN pure standard | Caco-2 | PC, NRU and MTS assays | 0.3–40 µg/mL for 24, 48 h | The most significant endpoint was MTS assay. This endpoint revealed significant cytotoxicity in Caco-2 cells exposed to all concentrations assayed except for the lowest concentration after 24 h. The EC50 were 2.5 µg/mL for 24 h and 0.6 µg/mL for 48 h. | [ |
| Commercial CYN pure standard | HUVEC | PC, NRU and MTS assays | 0.3–40 µg/mL for 24, 48 h | The higher cytotoxic effects were observed in NRU. Very low rates of cell viability were reported at 40 µg/mL, being 20% and 3% after 24 and 48 h, respectively. Similarly, low EC50 were found, 1.5 µg/mL for 24 h and 0.8 for 48 h. | [ |
| Commercial CYN pure standard | Primary rat hepatocytes | Alarm blue assay | 10–360 nM for 24, 48 h | CYN reduced cell viability in hepatocytes exposed to 90, 180 and 360 nM CYN. The two higher concentrations (180 and 360 nM) decreased cell viability around 50% after 48 and 24 h, respectively. | [ |
| Commercial CYN pure standard | Caco-2 and Clone 9 cells | Alarm blue assay | 0.1–10 µM for 8, 10, 12, 24, 48, 72 h | No cytotoxicity was observed for Caco-2 cells exposed to CYN up to 72 h. However, a time and concentration-dependent decrease in viability of Clone 9 cells exposed to CYN in comparison to the controls. | [ |
| Commercial CYN pure standard | Primary human T-lymphocytes | FAM caspase activity kit | 1 µg/mL for 6, 24, 48 h | The viability of human T-lymphocytes decreased in a concentration and time dependent way. Significant decreases were observed in exposure to 1 µg/mL, with the highest alterations observed after 24 h of exposure. | [ |
| Purified extract containing CYN | HepG2 | NRU and MTT assay | 0.001–100 µg/L for 4, 12, 24, 48 h | CYN was not toxic to HepG2 cells after 48 h of exposure, except for the higher concentration (100 µg/L) with a decrease of 11%. At concentrations bellow 10 µg/L cell viability increased. | [ |
| Synthetic CYN analogues (11a, 11b, 11c and 22), 1 and guanidinoacetate (GAA) | human neutrophils | MTT assay | 2.0 μg/mL for 1 h | The general toxicity decreased in the following order: 11c > 11a > 1 > 11b > 22 > GAA. No remarkable toxic effect was observed for the two last compounds (22 and GAA). | [ |
Abbreviations: BE-2 (Caucasian bone-marrow neuroblastoma cell line); Caco-2 (human colorectal adenocarcinoma cell line); CHO (Chinese hamster ovary cell line); CHO (a subclone from the parental CHO cell line); cylindrospermopsin (CYN); C3A (human hepatocellular carcinoma); effective mean concentration (EC50); guanidinoacetate (GAA); HCT-8 (human ileal adenocarcinoma); HDF (human dermal fibroblast cell line); HepG2 (human liver hepatocellular carcinoma cell line); HuTu-80 (human duodenal adenocarcinoma); HUVEC (human vascular endothelium cell line); IC50 (inhibitory mean concentration); KB (human cervix carcinoma); MNA (mouse neuroblastoma cell line); MTS (3-(4,5-dimethylthiazol-2-yl)-5-(3-carboxymethoxyphenyl)-2-(4-sulfophenyl)-2H-tetrazolium); MTT (3-(4,5-dimethylthiazol-2-yl)-2,5 diphenyltetrazolium bromide); NCI-N87 (human gastric carcinoma); PLHC-1 (Poeciliopsis lucida hepatocellular carcinoma cell line); SHE (Syrian hamster embryo cell line); Vero (African green monkey kidney).
In vitro morphological studies dealing with CYN.
| Toxin/Cyanobacteria | Experimental Model | Microscopy Used | Exposure Conditions Concentration Ranges | Main Results | Reference |
|---|---|---|---|---|---|
| Purified extract containing CYN and deoxyCYN | HepG2, BE-2 and MNA cells | Light microscope | 0.5–5 µg/mL for 24, 48 h | The BE-2 and MNA cells underwent shrinkage and cell rounding at 2.5 and 5 µg/mL, respectively. These findings indicated apoptosis process. | [ |
| Commercial CYN pure standard | SHE cells | Light microscope | 1 × 10−7–1 × 10−3 ng/mL for 7 days | CYN induced morphological cell transformation after 7 days of treatment with CYN (1 × 10−7–1 × 10−2 ng/mL), with nuclear enlargement. The morphologically transformed phenotype also showed loss of contact inhibition and density-dependent inhibition of cells. | [ |
| Commercial CYN pure standard | Caco-2 cells | Light and electron microscopes | 0.625, 2.5 µg/mL for 24, 48 h | The most remarkable ultrastructural changes were lipid degeneration, mitochondrial damage and nucleolar segregation with altered nuclei. | [ |
| Commercial CYN pure standard | HUVEC cells | Light and electron microscopes | 0.3–40 µg/mL for 24, 48 h | The main findings observed were nucleolar segregation with altered nuclei, degenerated Golgi apparatus, increases in the presence of granules and apoptosis. | [ |
| Commercial CYN pure standard | Clone 9 cells | Light microscope | 5 µM for 24, 48 h | After 24 h of treatment with CYN no discernible effect was observed, although after 48 h signs of damage and detachment of cells were reported. | [ |
Abbreviations: BE-2 (Caucasian bone-marrow neuroblastoma cell line); Caco-2 (human colorectal adenocarcinoma cell line); Clone 9 (Rattus norvegicus epithelial liver cell line); cylindrospermopsin (CYN); deoxycylindrospermopsin (deoxyCYN); HepG2 (human liver hepatocellular carcinoma cell line); HUVEC (human vascular endothelium cell line); MNA (mouse neuroblastoma cell line); SHE (Syrian hamster embryo cell line).
In vitro toxicokinetics studies performed with CYN.
| Toxin/Cyanobacteria | Experimental Model | Assays Performed | Exposure Conditions Concentration Ranges | Main Results | Reference |
|---|---|---|---|---|---|
| Commercial CYN pure standard | Primary rat hepatocytes and KB cells | Incubation with cholate and taurocholate and measurement of CYN uptake across hepatocyte | 800 ng/mL for 0, 24, 48, 72 h | There was no protection against the toxicity of CYN at 72 h by both bile acids, although some protection was observed after 48 h. This suggests that bile acid transport may be involve in certain extent in the uptake of the toxin. | [ |
| Commercial CYN pure standard | Vero-GFP cells | Monitoring CYN uptake in Vero cells expressing green fluorescent protein (GFP) | 0.1–100 µM for 4, 24 h | CYN effects on GFP signal increased 6 fold over 4–24 h incubation indicating slow, progressive uptake of the toxin. However, the mechanism involved was not elucidated. | [ |
| Commercial CYN pure standard | Caco-2 cells | Study of intestinal permeability of CYN | 1–10 µM for 3, 10, 24 h | The CYN uptake across Caco-2 cells is limited. Only 2.4–2.7% of CYN was detected in the basolateral side after 3 h, increasing slightly up to 16.7–20.5% after 24 h. | [ |
| Commercial CYN pure standard | HepG2 cells | Study the influence of cytochrome P450 (CYP) inductors on the cytotoxicity of CYN by means of viability assays | 1, 10 µg/L for 4, 12, 24, 48 h | CYPs induction made HepG2 cells more sensitive to CYN toxic effects. Moreover, low concentrations of CYN increased the metabolism in HepG2 cells. | [ |
| Commercial CYN pure standard | HepaRG cells and liver tissue fractions | Study of the metabolism of CYN by means of neutral red uptake assay with and without ketaconazol as well as by measuring CYN by LC/MS | 0.1–50 µM for 24 h | The use of ketoconazole, a CYP3A4 inhibitor, led to a decreased cytotoxicity of CYN. However, no decrease of CYN was reported after co-incubation with the inhibitor both in HepaRG and liver fractions measured by high resolution mass spectrometry. | [ |
| Commercial CYN pure standard | Caco-2 cells | Study of intestinal transport of CYN | 0.8 mg/L for 30, 60, 90, 120 min | The paracellular route was pointed out as the most important pathway in CYN absorption. Although a second mechanism was not identified, some insights were reported. This minor carrier-mediated transcellular transport may be independent of energy and Na+ and dependent of H+ and GSH. | [ |
Abbreviations: Caco-2 (human colorectal adenocarcinoma cell line); cylindrospemopsin (CYN); HepaRG: (human hepatoma cells); HepG2: (human hepatoma cells); KB (human cervix carcinoma); Vero (African green monkey kidney).
In vitro oxidative stress studies dealing with CYN exposure.
| Toxin/Cyanobacteria | Experimental Model | Assays Performed | Exposure Conditions Concentration Ranges | Main Results | Reference |
|---|---|---|---|---|---|
| Purified extract from | Primary rat hepatocytes | GSH | 0.8–5 µM CYN for 18 h. | 1.6 µM CYN caused a significant fall (~50%) in cell GSH. At 5 µM GSH cell was only 12.5%. The fall in GSH preceded an increase in LDH release. Reduction of GSH contributes to toxicity. Potentiating effects were found when cells were exposed to CYN and PPG. GSH is most likely to be involved in the detoxification of CYN | [ |
| Purified extract from | Primary rat hepatocytes | GSH | 0, 2.5, 5 µM CYN. Different exposure times depending on the experiment | GSH was depleted significantly after 16 h exposure to 2.5 µM CYN and after 10 h to 5 µM. CYN caused a C-dependent inhibition in GSH accumulation. There was no effect on GSH efflux. GSH synthesis was not altered by 2.5 µM CYN in cell free extracts but the high dilution of the cytosolic content (~500-fold) could avoid the detection of the GSH synthesis inhibition. Authors considered that the inhibition of GSH synthesis is the predominant mechanism for the CYN-induced fall in GSH. | [ |
| Purified extract from | Primary rat hepatocytes | GSH | 0, 0.16, 0.32, 0.63, 1.25, 2.5 and 5 µM natural CYN and CYN-DIOL | GSH IC50 values for CYN and RAC-CYN were 2.38 and 8.99 µM, respectively. When the racemic nature of RAC-CYN and the uncertainty in the original amounts of the synthetic analogues are taken into account, the decrease in GSH by RAC-CYN is almost equivalent to that of natural CYN. CYN-DIOL was as potent as CYN in lowering GSH levels, with the IC50 at 2.33 µM. Hepatocytes incubated with 6.25 µM EPI-CYN and EPI-DIOL had cell GSH levels of 39 ± 2.5 and 66 ± 14% of control respectively. | [ |
| Purified extract from | Primary mouse hepatocytes | GSH | GSH: 0, 1, 5 µM | GSH levels were depleted by CYN concentrations of 1 μM and above after a 18-h exposure, and 5 μM produced a significant reduction after 10 h with almost complete depletion after 18 h. However, 5 μM CYN did not elevate levels of lipid peroxidation, as measured by MDA production, and furthermore, inhibition of glutathione reductase by BCNU did not increase MDA production. | [ |
| Commercial CYN pure standard | PLCH-1 cells derived from a hepatocellular carcinoma of the topminnow | ROS | 0, 2, 4 and 8 mg/mL for 24 h | ROS content increased in a C-dependent way. GSH and GCS activity showed a similar pattern: a significant increase at lowest concentration and a significant reduction at the highest one. The initial increase is considered a try to face the toxic insult. The depletion of GSH may be due to an inhibition of its synthesis. | [ |
| Purified extract containing CYN | RONS | 0.1, 1.0 or 10 µg/L for 72 h | Cells exposed to the all concentrations of CYN have similar GST and G6PDH activities in comparison to the control group. However, GST activity of the hepatocytes exposed to 10 µg/L was 12% lower than of those exposed to 1 µg/L. G6PDH showed a similar pattern with significant differences between CYN treated cells but not in comparison to the control. No significant alterations were observed for GSH concentration and also for the 2GSH/GSSG ratio. RONS increased 25% in all CYN-exposed groups. PCO did not change. LPO increased in all CYN-exposed groups. | [ | |
| Commercial CYN pure standard | Human intestinal Caco-2 cell line | ROS | 0, 0.625, 1.25 and 2.5 µg/mL for 24 h | ROS content was significantly increased only at the concentration of 1.25 mg/mL CYN. GSH and GCS activity were only significantly increased at 2.5 mg/mL. The decrease of ROS at the highest concentration can be related to the higher GSH levels due to its higher synthesis. | [ |
| Commercial CYN pure standard | Human vascular endothelium (HUVEC) | ROS | 0, 0.375, 0.75 and 1.5 µg/mL for 24 h | When HUVEC cells were exposed to 0.375 µg/mL CYN, ROS content was significantly enhanced, while at higher concentrations it decreased to the levels of the control group. GCS activity increased at the highest concentrations (0.75 and 1.5 µg/mL) with enhancements of 2.25 and 3.5-folds, respectively. GSH content underwent concentration-dependent enhancements, with a 3-fold increase at the highest concentration used in comparison with the control group. The recovery of basal ROS content can be related to the concentration-dependent increase in the GSH and the GCS activity observed. | [ |
| Commercial CYN pure standard | Human hepatoma cells HepG2 | ROS | 0.05, 0.1 and 0.5 µg/mL for 5 h | A C-dependent statistically significant increase of ROS was observed in cells treated with 0.05, 0.1 and 0.5 µg/mL CYN already after 30 min of exposure, which steadily increased with incubation time. After 5 h incubation, the fluorescence intensity at the highest dose of CYN was about five times higher than in the control cells. | [ |
| Commercial CYN pure standard | Primary rat hepatocytes | ROS | 0, 90, 180, 360 nM CYN for 24 and 48 h | CYN induced oxidative stress at all the concentrations tested after 24 and 48 h of incubation. A 3-fold increase in fluorescence was observed in hepatocytes treated with 360 nM CYN for 48 h. Resveratrol partially rescued the cells in a concentration dependent manner after 24 and 48 h of treatment. The increase in cell viability in cultures treated with CYN plus 20 μM resveratrol was about 32% and 7% after 24 and 48 h, respectively, when compared to that of CYN treated cells. A higher level of Nrf2 (transcription factor that regulates the expression of antioxidant enzymes) in toxin treated cells after 48 h was observed. | [ |
| Commercial CYN pure standard | Rat hepatic cell line, Clone 9 | GSH | 1 µM or 5 µM CYN for 4, 12, 24 and 48 h | Both treatments with CYN (1 and 5 mM) showed a clear and gradual increase of the GSH levels over time, especially at 48 h. No significant changes were observed on GCS level over time in cells exposed to 1 mM. 5 mM CYN, on the contrary, clearly increased levels of GCS time-dependently. | [ |
| Commercial CYN pure standard | ROS | 0, 0.1, 0.5 or 1 μg/mL for 3.5 h | A CYN-induced increase of ROS in exposed CLC cells was observed at each toxin concentration. The results were concentration dependent, with a growing tendency observed until the end of the experiment. In cells exposed to the lowest CYN concentration (0.1 μg/mL) SOD activity was elevated in a statistically significant manner, reaching 179% of the enzyme activity detected in the control cells. At the other tested CYN concentrations SOD activity was also slightly enhanced, however, these increases were not statistically significant. The toxin at each tested concentration increased the total GSH content in the cells, with the concomitant reduction of the GSH/GSSG ratio. | [ | |
| Purified extract from | Human hepatoma cells HepG2 | ROS | 0, 0.001, 0.01, 0.1, 1, 10 and 100 µg/L CYN for 48 h with 10% FBS | No concentration-dependent changes in superoxide production by the mitochondria, ROS and LPO. Actually, LPO decreased. GST activity only increased significantly at 100 µg/L. The 10% FBS could reduced toxicity. | [ |
| Commercial CYN pure standard | Human lymphocytes | ROS | 0, 0.01, 0.1 and 1 µg/mL CYN for 0.5–48 h to evaluate ROS production | CYN elevated ROS level in a concentration-dependent manner. The increase was observed within a time as short as 0.5 h of exposure and reached its maximum after 3 and 6 h. | [ |
| Purified extract from | ROS | 0, 0.1, 1.0, 10, and 100 μg/L for 72 h | The activities of SOD, CAT, GPx, GST and G6PDH were not altered by the exposure to CYN in all groups tested. Non-protein thiols concentration increased 72% only in the cells exposed to the highest CYN concentration. CYN caused a concentration-dependent decrease of GR activity in the cells exposed to >1.0 μg/L. ROS levels increased 40% only in the cells exposed to the highest CYN concentration. No significant damage to lipids (peroxidation), and proteins (carbonylation) was observed. | [ | |
| CYN | Human neutrophils | ROS | ROS: 2 µg/mL for 5–60 min | All the compounds tested had the ability to temporarily increase the intracellular ROS levels to different extents. LPO levels were significantly increased. | [ |
Abbreviations: BCNU: 1,3-bis(chloroethyl)-l-nitrosourea; CAT: Catalase; CYP: cytochrome P450; G6PDH: Glucose-6-phosphate dehydrogenase; FBS: Fetal Bovine Serum; GCS: Gamma Glutamylcysteine Synthetase; G6PDH: glucose-6-phosphate dehydrogenase; GPx: glutathione peroxidase; GR: Glutathione Reductase; GSH: Glutathione; GST: Glutathione S-transferase; GSSG-Rd: Glutathione disulfide reductase; LPO: Lipid peroxidation; MDA: Malondialdehyde; PCO: Protein carbonylation; PPG: Propargylglycine; RONS: Reactive oxygen/nitrogen species; ROS: Reactive Oxygen Species; SOD: Superoxide dismutase.
In vitro mutagenicity and genotoxicity studies performed with CYN.
| Toxin/Cyanobacteria | Experimental Models | Assays Performed | Exposure Conditions Concentration Ranges | Main Results | Reference |
|---|---|---|---|---|---|
| Purified extract from freeze-dried | Human lymphoblastoid cell line WIL2-NS | Cytokinesis-block micronucleus (CBMN) assay. Micronuclei (MN) were counted in binucleated cells (BNCs) | 1,3,6, and 10 µg CYN/mL, 24 h and 48 h | CYN induced significant increases in the frequency of MN in BNCs exposed to 6 and 10 µg/mL, and a significant increase in centromere (CEN)-positive MN at all concentrations tested. At the higher concentrations, both CEN-positive and CEN-negative MI were induced. | [ |
| Purified extract from a | Chinese hamster ovary K1 (CHO-K1) cells | Comet assay | 0.5–1.0 µg CYN/mL, 24 h | No significant induction of DNA strand breaks could be detected after 24 h treatment. However, cell growth was inhibited, as well as cell blebbing and rounding. | [ |
| Purified extract from | Primary mouse hepatocytes | Comet assay | 0.05–0.5 µM CYN. | CYN induced increases in comet tail length, area and tail moment at 0.05 µM. The CYP450 inhibitors completely inhibited the genotoxicity of CYN. | [ |
| Purified extract from | Human dermal fibroblasts (HDFs), Caco-2, HepG2 and C3A cells | Quantification of mRNA levels for selected p53-regulated genes using qRT-PCR | 1, 2.5, or 5 µg/mL CYN for 6 h or 24 h | After 6 h exposure to CYN, concentration-dependent increases in mRNA levels were observed for the p53 target genes | [ |
| Purified extract from two cultures of | CHO-K1 cells | Chromosome aberration (CA) assay | 0.05–2 µg CYN/mL were assayed. DNA damage was determined after 3, 16 and 21 h of exposure and the assay was performed with and without metabolic activation (S9) | CYN with and without S9 had no significant influence on the frequency of CA. | [ |
| Commercial pure standard CYN (>98% purity) | Caco-2 and HepaRG cells, differentiated and undifferentiated cells | Cytokinesis-block micronucleus (CBMN) assay | 0.5–2 µg CYN/mL, and the CYP450 inhibitor ketoconazole (1–5 µM) for 34 h | CYN increased the frequency of binucleated cells in both cell lines, and ketokonazole reduced both the genotoxicity and cytotoxicity induced by CYN | [ |
| Purified extract containing CYN | Hepatocytes of the fish | Comet assay | 0.1, 1.0, or 10 µg CYN/L for 72 h | No significant effects on DNA strand breaks were found. | [ |
| Commercial pure standard CYN | HepG2 cell line (human hepatoma cell line) | Comet assay, and MN, nuclear bud (NBUD), nucleoplasmic bridge (NPB) formation. | 0–0.5 µg CYN/mL) for 4, 12, and 24 h | Non cytotoxic concentrations of CYN (0–0.5 µg/mL) induced increased DNA strand breaks after 12 and 24 h of exposure. Increased frequency of MN, NBUDs and NPBs after 24 h exposure in a dose-dependent manner was reported. CYN upregulated the expression of the | [ |
| Commercial pure standard CYN | Human peripheral blood lymphocytes (HPBLs) | Comet assay and the cytokinesis-block micronucleus (CBMN) assay. Gene expression of | The whole blood was treated with CYN (0, 0.05, 0.1 and 0.5 μg/mL) for the comet and CBMN assays. For the mRNA expression the isolated HPBLs were exposed to 0.5 μg/mL of CYN for 4 and 24 h | In HPBLs CYN induced the formation of DNA single strand breaks (comet assay), a time and dose-dependent increase in the frequency of MN and NBUD was observed, and a slight increase in the number of NPB. CYN up-regulated the genes | [ |
| Commercial pure standard CYN and crude extracts from cyanobacterial blooms. Mixture of commercial pure toxins: CYN, MC-LR and anatoxin-a | Mutagenicity: Ames test | Pure CYN: 0.312, 0.625, 1.25, 2.5, 5 and 10 µg/mL. The mixture of pure toxins (CYN, MC-LR and anatoxin-a) at 1 µg/mL was also tested but only in two | Mutagenicity was detected in four of the ten extracts assayed, mainly against | [ | |
| Commercial CYN Pure standard | Common carp ( | Alkaline version of comet assay | 0.5 µg CYN/mL for 18 h | The cells treated with CYN were affected to a lesser extent in comparison to the damage induced by MC-LR. | [ |
| Commercial CYN Pure standard | HepG2 cell line (human hepatoma cell line) | Formation of double strand breaks (DSBs). Analysis of the cell-cycle by flow-cytometry | 0–0.5 µg CYN/mL for 24–96 h | CYN induced formation of DSBs after 72 h exposure. The toxin has impacts on the cell cycle, indicating G0/G1 arrest after 24 h and S-phase arrest after longer exposure (72 and 96 h). | [ |
| Commercial CYN Pure standard | HepG2 cells | Gene expression was analyzed by qPCR | 0.5 µg CYN/mL for 12 and 24 h | CYN increased expression of the immediate early response genes, and strong up-regulation of the growth arrest and DNA damage inducible genes ( | [ |
| Commercial CYN Pure standard | HepG2 cells | Alkaline comet assay and Fpg -enzyme modified assay | 0–0.5 µg CYN/mL) for 4, 12 and 24 h | No DNA damage was observed after 4 h exposure to CYN. After 12 and 24 h, CYN (0.25–0.50 µg/mL) induced significant increase of DNA strand breaks, but not oxidative damage. CYN did not induce apoptosis. | [ |
| Treated water; crude extract of | HepG2 cells | Comet assay | Cells were exposed to all extracts at concentration of 0.1, 0.5 and 1 µg of dry material/mL, and also to treated water only, for 24, 48 and 72 h | DNA damage was detected only under toxic | [ |
| Commercial CYN Pure standard | HepG2 cells with a plasmid that encodes the fluorescent protein DsRed2 under the control of the | The induction of the DsRed fluorescence intensity was determined by spectrofluorimetry, fluorescence microscopy and flow cytometry | Cells were exposed to CYN and the DsRed fluorescence was determined at 24 and 48 h of exposure; the cell viability was determined at 48 h | LOEC 2: 0.12 μM and RDF 3: 1.53 μM | [ |
| Commercial CYN Pure standard | The cytokinesis-block micronucleus (CBMN) assay. The fluorimetric OxyDNA assay kit was also employed | 0.1, 0.5, or 1 µg CYN/mL, for 24 h | CYN increase the number of MN, and oxidative DNA damage was also detected. | [ | |
| Commercial CYN and MC-LR pure standards, and mixtures MC-LR/CYN | HepG2 cells | Alkaline comet and CBMN assays were performed. The expression of selected genes was analyzed by quantitative time PCR | CYN: 0.01–0.05 µg CYN/mL; MC-LR: 1 µg/mL, and MC-LR/CYN mixtures for 4 h and 24 h | CYN after 24 of exposure induced DNA stand breaks and genomic instability. The MCLR/CYN mixture induced DNA strand breaks after 24 h exposure, but to a lesser extent as CYN alone. The induction of genomic instability and changes in the expression of selected genes induced by the mixture were similar to those induced by CYN alone. | [ |
| Purifies extract from the strain | Comet assay | 0.1–100 µg/L of CYN for 72 h | No significant DNA damage was observed | [ |
1 Fpg: Formamidopyrimidine glycosylase enzyme; 2 LOEC: Lowest effective concentration that induced ≥1.5-fold increase in relative DsRed fluorescence, over the solvent-treated control; 3 RDF: Relative DsRed fluorescence induction detected at LOEC.