Microcystic Cyanobacteria Extract Induces Cytoskeletal Disruption and Intracellular Glutathione Alteration in Hepatocytes.Microcystins are a group of highly liver-specific toxins, although their exact mechanisms of action remain unclear. We examined the effects of microcystic cyanobacteria cyanobacteria (sī'ənōbăktĭr`ēə, sī-ăn'ō–) or blue-green algae, photosynthetic bacteria that contain chlorophyll. extract (MCE See Media Center Edition. ) collected from a contaminated water source on the organization of cellular microtubules Microtubules Slender, elongated anatomical channels in worms. Mentioned in: Antihelminthic Drugs (MTs) and microfilaments microfilaments, n.pl any of the submicroscopic cellular filaments, such as the tonofibrils, found in the cytoplasm of most cells, that function primarily as a supportive system. (MFs) in hepatocytes. We also investigated the effects on lactate dehydrogenase (LDH LDH -lactate dehydrogenase. LDH abbr. lactate dehydrogenase LDH lactic acid dehydrogenase; see lactate dehydrogenase. ) leakage and intracellular glutathione (GSH GSH reduced glutathione. GSH reduced glutathione. ). Primary cultured rat hepatocytes exposed to MCE (equivalent to 125 [micro]g/mL lyophilized ly·oph·i·lize tr.v. ly·oph·i·lized, ly·oph·i·liz·ing, ly·oph·i·liz·es To freeze-dry (blood plasma or other biological substances). [lyophil(ic) + -ize. algae algae (ăl`jē) [plural of Lat. alga=seaweed], a large and diverse group of primarily aquatic plantlike organisms. These organisms were previously classified as a primitive subkingdom of the plant kingdom, the thallophytes (plants that cells) showed a characteristic disruption of MTs and MFs in a time-dependent manner. Under these conditions, MCE caused aggregation of MTs and MFs and a severe loss of MTs in some cells. Moreover, MCE-induced cytoskeletal cy`to`skel´e`tal a. 1. (Cell Biology) Of or pertaining to the cytoskeleton; as, cytoskeletal microtubules s>. alterations preceded the LDH leakage. On the other hand, the treatment of cells with MCE led to a dose-dependent increase of intracellular GSH. However, time-course study showed a biphasic bi·pha·sic adj. Having two distinct phases: a biphasic waveform; a biphasic response to a stimulus. change of intracellular GSH levels with a significant increase in the initial stage followed by a decrease after prolonged treatment. Furthermore, pretreatment pretreatment, n the protocols required before beginning therapy, usually of a diagnostic nature; before treatment. pretreatment estimate, n See predetermination. with N-acetylcystein (NAC See network access control. ), a GSH precursor, significantly enhanced the intracellular GSH level and decreased the MCE-induced cytotoxicity as well as cytoskeleton cytoskeleton System of microscopic filaments or fibres, present in the cytoplasm of eukaryotic cells (see eukaryote), that organizes other cell components, maintains cell shape, and is responsible for cell locomotion and for movement of the organelles within it. changes. In contrast, buthionine-(S,R)-sulfoximine, a specific GSH synthesis inhibitor, increased the cell susceptibility to MCE-induced cytotoxicity by depleting the intracellular GSH level. These findings suggest that intracellular GSH plays an important role in MCE-induced cytotoxicity and cytoskeleton changes in primary cultured rat hepatocytes. Increasing intracellular GSH levels protect cells from MCE-induced cytotoxicity and cytoskeleton changes. Key words: cyanobacteria, cytoskeleton, glutathione, hepatocytes, hepatotoxicity hepatotoxicity (hepˑ·  ·tō·t , microcystin. Environ Health Perspect 108:605-609 (2000). [Online 25 May 2000] http://ehpnet1.niehs.nih.gov/docs/2000 /108p605-609ding/abstract.html The occurrence of heavy freshwater blooms of cyanobacteria (blue-green algae) has been well reported in many parts of the world (1). Among the toxic blue-green algae, Microcystis is the most common genera producing microcystins, a group of toxins with strong hepatotoxicity (1,2). These toxins are able to cause the death of domestic and wild animals as well as human illness (3). Recently, it has been reported that dialysis patients in Brazil died of acute hepatic failure due to cyanobacteria contamination of the water used for dialysis (4,5). Recent epidemiologic studies have suggested that the cyanobacteria-contaminated water could be related to the high incidence of primary liver cancer in certain areas of China (6,7). Our previous study also showed that microcystic cyanobacteria extract (MCE) of a water source in China had potent genotoxicity Genotoxic substances are a type of carcinogen, specifically those capable of causing genetic mutation and of contributing to the development of tumors. This includes both certain chemical compounds and certain types of radiation. (8). Microcystins are highly liver specific and their hepatotoxicity has been well studied (9-11). However, the exact mechanisms by which microcystins cause hepatotoxicity have not been fully elucidated. One of the extensively studied mechanisms is that microcystins are potent inhibitors of protein phosphatase 1 and 2A, which lead to the increase of protein phosphorylation phosphorylation, chemical process in which a phosphate group is added to an organic molecule. In living cells phosphorylation is associated with respiration, which takes place in the cell's mitochondria, and photosynthesis, which takes place in the chloroplasts. (1). The hyperphosphorylation of proteins have been attributed to the destruction of intermediate filaments (IFs) (12,13). Microcystin-disrupted microfilaments (MFs) have 'also been reported (14,15). In contrast, only one study showed that microtubules (MTs) were disrupted by microcystin-LR in primary cultured rat hepatocytes and several nonhepatocyte cell lines (16). However, at present, there are no studies to show that MF and MT proteins have also been phosphorylated by microcystin. Therefore, it is possible that there is another mechanism, besides protein phosphorylation, which contributes to microcystin-disrupted MFs and MTs. The cytoskeleton consists of three major structural elements: MTs, MFs, and IFs. These elements play an important role in maintaining cellular architecture and internal organization, cell shape, motility motility /mo·til·i·ty/ (mo-til´ite) the ability to move spontaneously.mo´tile Motility Motility is spontaneous movement. , cell division, and many other processes (17). There are many cysteine cysteine (sĭs`tēn), organic compound, one of the 20 amino acids commonly found in animal proteins. Only the l-stereoisomer participates in the biosynthesis of mammalian protein. residues in the cytoskeleton proteins, and certain tubulin-SH groups are crucial for its polymerization polymerization Any process in which monomers combine chemically to produce a polymer. The monomer molecules—which in the polymer usually number from at least 100 to many thousands—may or may not all be the same. in vitro (18). Cellular-reduced glutathione (GSH) is important for the regulation of cytoskeleton organization (19). Perturbing the cellular redox redox (rē`dŏks): see oxidation and reduction. status by depleting intracellular GSH provoked disruption of MFs in human fibroblasts Fibroblasts A type of cell found in connective tissue; produces collagen. Mentioned in: Skin Grafting (20). It has been reported that certain metal carcinogens such as cadmium and arsenite disrupted cytoskeletal structures, and those changes had a close relationship with the cellular GSH level alterations (21,22). At present, there are several lines of evidence suggesting that GSH may play a critical role in the detoxification of microcystins. Microcystins could conjugate with GSH in cell-free systems or in the liver tissue in vivo (23-25), which substantially reduced its cytotoxicity (23). Moreover, our previous studies showed that MCE induced lipid peroxidation and reactive oxygen species reactive oxygen species, n molecules and ions of oxygen that have an unpaired electron, thus rendering them extremely reactive. Many cellular structures are susceptible to attack by ROS contributing to cancer, heart disease, and cerebrovascular disease. (ROS ROS, n.pr See reactive oxygen species. ) formation in primary cultured rat hepatocytes (26,27), suggesting the possible effect of MCE on cellular redox status. However, so far there is no systematic study on the role of GSH in the hepatotoxicity of microcystins and its association with the cytoskeleton. Thus, in the present study, we aimed to determine the involvement of GSH on the MCE-induced cytotoxicity and disruption of MTs and MFs in primary cultured hepatocytes. In our study, the intracellular GSH level in rat hepatocytes was modulated by N-acetyl-cystein (NAC), a GSH precursor, and buthionine-(S,R)-sulfoximine (BSO BSO Bilateral salpingo-oophorectomy. Excision of both ovaries ), a specific GSH synthesis inhibitor. Data from these experiments provide direct evidence showing that GSH is closely involved in MCE-induced cytoskeletal disruption and hepatotoxicity. Materials and Methods Chemicals. We purchased William's medium E, insulin, collagenase collagenase /col·la·ge·nase/ (kah-laj´e-nas) an enzyme that catalyzes the hydrolysis of peptide bonds in triple helical regions of collagen. col·lag·e·nase n. , Hepes, L-glutamine, penicillin, and streptomycin, NAC, BSO, GSH, o-phthalaldehyde (OPT), and mouse fluorescein isothiocyanate (FITC FITC fluorescein isothiocyanate; used as a fluorescent label for proteins, especially antibodies. ) conjugate monoclonal anti-[Beta]-tubulin from Sigma (St. Louis, MO). We purchased fetal bovine serum Fetal bovine serum ( or foetal bovine serum) is serum taken from the fetuses of cows. Fetal Bovine Serum (or FBS) is the most widely used serum in the culturing of cells. In some papers the expression foetal calf serum is used. (FBS FBS abbr. fasting blood sugar FBS Fasting blood sugar. See Fasting glucose. ) from Gibco BRL BRL In currencies, this is the abbreviation for the Brazilian Real. Notes: The currency market, also known as the Foreign Exchange market, is the largest financial market in the world, with a daily average volume of over US $1 trillion. (Life Technologies, Gaithersburg, MD) and Alex 488 phalloidin phalloidin /phal·loi·din/ (fah-loid´in) a hexapeptide poison from the mushroom Amanita phalloides, which causes asthenia, vomiting, diarrhea, convulsions, and death. phal·loi·din n. and propidium iodide (PI) from Molecular Probes (Eugene, OR). All other common chemicals were reactive agent grade and were purchased from Merck (Darmstadt, Germany). Sampling of cyanobacteria. In early fall 1995 we collected the blue-green algae from Dianshan Lake, one of the main water supply sources for Shanghai, during a water bloom period. Shanghai is the largest city in the People's Republic of China. The water blooms were dominated by Microcystis aeruginosa (determined by microscopic examination) and the algae cells were lyophilized for toxins extraction. Extraction of toxins. We extracted the toxins as described by Ding et al. (8). Briefly, we suspended lyophilized algae cells (25 mg) in 2.5 mL n-butanol:methanol:water (1:4:15, v/v/v), then the suspension was centrifuged at 16,000g for 30 min. The supernatant from three extractions was pooled together and then passed through a preconditioned SepPak C18 cartridge (3 mL tube; Supelco, Bellefonte, PA) to eliminate some impurities by washing with 3 mL 20% methanol, then eluted with 10 mL pure methanol. Finally, the methanol elute e·lute tr.v. e·lut·ed, e·lut·ing, e·lutes To extract (one material) from another, usually by means of a solvent. [From Latin was evaporated to dryness at 56 [degrees] C and dissolved in 2 mL distilled and deionized water. Liver perfusion and primary rat hepatocyte hepatocyte /hep·a·to·cyte/ (hep´ah-to-sit?) a hepatic cell. hep·a·to·cyte n. A parenchymal liver cell. Hepatocyte A liver cell. culture. Liver perfusion and primary rat hepatocyte culture were carried out as reported earlier (27). The cells were plated at a density of 4 x [10.sup.6] cells/75 [cm.sup.2] flask (Corning, Stony Brook, NY). After preincubation for 2 hr in 10 mL complete Williams' medium E (supplemented with 2 mM L-glutamine, 0.02 IU insulin/mL, and 10% FBS), we washed the flasks with prewarmed Hepes buffer (pH 7.4) to remove the unattached dead cells. The hepatocytes were then incubated in serum-free Williams' medium E with various treatments. Treatments. For the dose-response study, we incubated cells with three doses of MCE for 6 hr: the low concentration (equivalent to 1.25 [micro]g lyophilized algae cells/mL, the moderate concentration (equivalent to 12.5 [micro]g lyophilized algae cells/mL, and the high concentration (equivalent to 125 [micro]g lyophilized algae cells/mL). For the time-course study, we exposed hepatocytes to high concentration of MCE (125 [micro]g lyophilized algae cells/mL) for designated periods of time. To study the role of GSH in modulating MCE-induced cytotoxicity, we pretreated cells with NAC 10 mM or BSO 2.5 mM for 6 hr, then washed them with Hepes buffer once. The cells were further exposed to the high concentration of MCE (125 [micro]g/mL for another 6 hr. We examined the cytotoxicity and intracellular GSH levels. Detection of cytoskeleton disruption. Primary hepatocytes on cover slides (12 x 12 mm) in 35-mm Petri dishes were preincubated for 2 hr in 5 mL Williams' medium E supplemented with 10% FBS, then washed with Hepes buffer once. We then incubated the hepatocytes in serum-free Williams' medium E with the high concentration of MCE for up to 6 hr. Both control and treated cells were processed for fluorescent staining for MT and MF visualization. To study the effects of NAC on MCE-induced MT and MF changes, we pretreated the cells with 10 mM NAC for 6 hr and washed them once with Hepes buffer. The cells were then exposed to MCE for another 6 hr. MFs were determined according to the protocol provided by the manufacturer (Molecular Probes) with certain modifications. Briefly, cells on cover slides were washed twice with phosphate-buffered saline (PBS PBS in full Public Broadcasting Service Private, nonprofit U.S. corporation of public television stations. PBS provides its member stations, which are supported by public funds and private contributions rather than by commercials, with educational, cultural, ) and then fixed with freshly prepared 3.7% paraformaldehyde paraformaldehyde: see formaldehyde. in PBS for 30 min. The cells were permeabilized with 0.1% Triton x 100 in PBS for 15 min and then blocked with 1% bovine serum albumin in PBS for 30 min at room temperature. The MFs and nuclei on cover slides were then stained with Alex 488 Phalloidin (1:40 dilution) and 10 [micro]g/mL PI, respectively. We labeled MTs according to Li and Chou (21), with modifications. Briefly, the cells were first washed with PBS and with a microtubule microtubule Tubular structure enclosed by a membrane found within animal and plant cells. Of varying length, they have several functions. They help give shape to many cells and are major components of cilia and flagella, participate in the formation of the spindle during stabilizing buffer (PM2G) containing 0.1 M Pipes, 1 mM Mg[SO.sub.4], 2 M glycerol glycerol, glycerin, glycerine, or 1,2,3-propanetriol (prō`pāntrī'ŏl), CH2OHCHOHCH2OH, colorless, odorless, sweet-tasting, syrupy liquid. , and 2 mM EGTA EGTA egtazic acid; a chelator similar in structure and function to EDTA (ethylenediaminetetraacetic acid) but with a higher affinity for calcium than for magnesium. (pH 6.9). The cells were fixed with freshly prepared 3.7% paraformaldehyde in PM2G for 30 min and washed with PBS once. The cells were then permeabilized with 0.5% NP-40 in PBS. MTs were labeled with mouse FITC conjugate monoclonal anti-[Beta]-tubulin (1:25 dilution) for 1 hr at room temperature. For both MF and MT staining, we mounted the coverslides on glass slides with a drop of mounting solution (PBS:glycerol, 3:1). We then examined the cytoskeletal morphologies with an Olympus confocal confocal see confocal microscopy. microscope (Olympus, Tokyo, Japan) equipped with a krypton/argon laser and an Olympus 60 x numerical aperture, 1.25 Planapo objective. Excitation intensity was set to provide bright pixels without saturation. Determination of cytotoxicity. We determined the cytotoxicity of MCE on cultured rat hepatocytes by the percentage of lactate dehydrogenase (LDH) leakage from cells into the medium (27), which was calculated according to the following formula: %LDH leakage = (LDH activity present in the medium after treatment/total LDH activity at the same time) x 100. Determination of intracellular GSH content. We determined the intracellular GSH content according to the method of Hissin and Hilf (28). The stock solution of the fluorescent probe OPT was freshly prepared in methanol (1 mg/mL). After various designated treatment, cells were collected using cell scrapers and washed twice with cold PBS and then suspended in 0.1 M sodium phosphate/5 mM EDTA EDTA: see chelating agents. (pH 8.0). After ultrasonication, we mixed 0.75 mL cell homogenate homogenate /ho·mog·e·nate/ (ho-moj´in-at) material obtained by homogenization. homogenate material obtained by homogenization. with 0.2 mL 25% metaphosphoric acid to precipitate the proteins. We monitored the fluorescence intensity of OPT with excitation wavelength at 350 nm and emission wavelength at 420 nm. We established a GSH calibration curve using standard GSH, and the GSH concentration was expressed as nanomole per [10.sup.6] cells. Statistical analysis. We repeated each experiment at least 3 times and the numerical data were presented as means [+ or -] SD and analyzed using Student's t-test. We considered a p-value [is less than] 0.05 statistically significant. Results MCE-induced dose- and time-dependent increase of LDH leakage. When we treated cells with MCE for 6 hr, there was no significant change of LDH leakage in the low (1.25 [micro]g lyophilized cells/mL) and the moderate concentration of MCE (12.5 [micro]g lyophilized cells/mD (Figure 1A). For cells treated with the high concentration of MCE (125 [micro]g lyophilized cells/mL), there was a significant increase of LDH leakage (p [is less than] 0.05). Figure 1B shows a time-dependent increase of LDH leakage when rat hepatocytes were treated with 125 [micro]g MCE for 24 hr. The LDH leakage was approximately 70% and the control group remained a constant low LDH leakage level (around 10%) at 24 hr. In our experiments, the total LDH activity is mainly dependent on the cell number added into each flask at the beginning of the treatment. The total LDH remained relatively stable under our experimental conditions in the relatively short culture time of our experiments. [Figure 1 ILLUSTRATION OMITTED] MCE-induced dose- and time-dependent alterations of intracellular GSH. A dose-dependent increase of intracellular GSH in MCE-treated hepatocytes is shown in Figure 2A. Figure 2A clearly shows that MCE increased the intracellular GSH level markedly after a 6-hr treatment with 12.5 and 125 [micro]g MCE (p [is less than] 0.05). In contrast, time-course studies showed that cells exposed to the high concentration of MCE (125 [micro]g lyophilized cells/mL) exhibited a biphasic response in their intracellular GSH. The intracellular GSH showed no significant change until 3 hr, when it started to increase sharply and reached the maximum level at 6 hr. After 12-hr treatment, the intracellular GSH level started to decrease but was still significantly higher than the control (p [is less than] 0.05). After 24-hr treatment, the intracellular GSH level reduced drastically (Figure 2B). Similar patterns of intracellular GSH level changes were also observed when GSH was measured using monochlorobine in flow cytometry (results not shown). [Figure 2 ILLUSTRATION OMITTED] Alterations in cytoskeletal organization. Figure 3 shows the morphologies of cells stained for MTs and MFs and nuclei. The normal hepatocytes contain a highly organized network of MTs that are distributed evenly in a wavy and curving pattern (Figure 3A). In hepatocytes treated with 125 [micro]g MCE, the filamentous pattern of MTs was disrupted and collapsed toward the interior of the cells after 1 hr treatment (Figure 3C). When treated with 125 [micro]g MCE for 3 hr, we observed a noticeable reduction in the number of MTs in the cells, whereas densely aggregated MTs appeared to retract around the nucleus. Moreover, in some cells all MTs were lost and only the nuclei were stained (Figure 3E, arrow). This effect was more evident when cells were treated for 6 hr (Figure 3G). In contrast, when cells were pretreated with NAC for 6 hr, the lost and aggregated MTs caused by MCE were significantly protected (Figure 3I). [Figure 3 ILLUSTRATION OMITTED] Figure 3B shows the normal MF organization in untreated cells. MFs in the untreated cells show uniform distribution and good organization. Exposure of cells to MCE (125 [micro]g/mL) for 1 hr produced severe MF disorganization disorganization /dis·or·gan·iza·tion/ (-or?gan-i-za´shun) the process of destruction of any organic tissue; any profound change in the tissues of an organ or structure which causes the loss of most or all of its proper characters. , characterized by the concentration of actin fibers inside the plasma membrane of some cells and the aggregation or collapse into the interior of the cells (Figure 3D). These rosettelike aggregates of actin fibers in some cells emerged from the cytoplasm and protruded into the blebs when the cells were treated with MCE for 3 hr (Figure 3F). After 6 hr treatment with MCE, we observed an obvious reduction of MFs (Figure 3H). However, much better organized MFs reappeared when the cells were pretreated with NAC for 6 hr (Figure 3J). We found similar morphologic changes of MTs and MFs when the hepatocytes were treated with pure microcystin-LR at 0.1 [micro]M (data not shown) Effects of NAC and BSO on MCE-induced cytotoxicity. To assess the role of GSH in modulating MCE-induced cytotoxicity, we pretreated cultured rat hepatocytes with NAC (10 mM) or BSO (2.5 mM) for 6 hr and washed them once with Hepes buffer. The cells were then further exposed to 125 [micro]g MCE for another 6 hr. Figure 4A shows the effects of NAC and BSO on MCE-induced cytotoxicity, as measured by the percentage of LDH leakage. NAC or BSO alone did not significantly cause the LDH leakage in rat hepatocytes. However, when cells were pretreated with NAC for 6 hr, the cytotoxicity induced by MCE was significantly reduced (p [is less than] 0.05). In contrast, when cells were pretreated with BSO, the LDH leakage was enhanced significantly as compared to cells treated with MCE only (p [is less than] 0.05). The results indicate that intracellular GSH protects the cells against MCE-induced cytotoxic effects, and depleting intracellular GSH leads to increased susceptibility to cell damage. [Figure 4 ILLUSTRATION OMITTED] We also investigated the effect of NAC and BSO pretreatment on MCE-induced intracellular GSH changes. Figure 4B shows that NAC enhanced the intracellular GSH level, whereas BSO decreased the intracellular GSH level. Furthermore, when cells were pretreated with NAC and MCE, there was a significant increase of intracellular GSH (p [is less than] 0.05). In contrast, we observed that the intracellular GSH level decreased significantly when cells were exposed to BSO and MCE (p [is less than] 0.05). Discussion In this study we have shown that hepatocytes exposed to MCE exhibit characteristic alterations in cytoskeletal morphology caused by the disappearance of regular filamentous structure soon after MCE treatment. We observed severe reorganization of MTs and aggregation of MFs after prolonged treatment. These results are in agreement with previous reports using pure microcystin-LR (14,16), and are in line with our earlier finding using MCE (26,27), where microsystin-LR was identified as the main component (8). Microcystin-LR is a strong inhibitor of protein phosphatase 1 and 2A and eventually causes hyperphosphorylation of cytosolic and cytoskeletal proteins (14). Phosphorylation is an important mechanism regulating the organization of cytoskeleton. The IFs proteins can be phosphorylated and the phosphorylation status is closely correlated with its disassembly (29). Toivola et al. recently reported that microcystin-LR induced hyperphosphorylation of keratin keratin (kĕr`ətĭn), any one of a class of fibrous protein molecules that serve as structural units for various living tissues. The keratins are the major protein components of hair, wool, nails, horn, hoofs, and the quills of feathers. 8 and 18, which eventually led to the disruption of IFs. In addition, phosphorylation of microtubule-associated proteins (MAPS) and actin-associated proteins may induce alterations of polymerization of MTs and distribution of MFs (30,31). However, it is still unclear at this stage whether the observed MT and MF changes induced by microcystin are a result of increased phosphorylation of MAPS with the subsequent destabilization of MTs and MFs. An earlier study showed that phosphorylation of tubulin tubulin /tu·bu·lin/ (too´bu-lin) the constituent protein of microtubules. tu·bu·lin n. A globular protein that is the structural constituent of microtubules. and MAPS was not changed by calyculin A, another potent inhibitor of protein phosphatase 1 and 2A (12), although the concentration used (50 nM) was relatively low. On the other hand, several studies suggested that oxidative stress could affect actin dynamics by markedly inhibiting the assembly of actin monomers and eventually disrupted its structure (32,33). In our earlier study, we showed that MCE could induce ROS formation in rat hepatocytes with a relatively short exposure time ([is less than] 1 hr) (27). Therefore, MCE-induced ROS formation may play an important role in the disruption of MF structure, as observed in the present study. In addition to the reorganization and aggregation of MTs induced by MCE in primary cultured rat hepatocytes, some cells lost MTs after MCE treatment. To our knowledge, this effect has not been previously reported in any cell type treated with microcystin. MTs are composed of [Alpha]- and [Beta]-tubulin subunits, which contain 12 and 8 cysteine residues, respectively (17). Cellular GSH acts as a buffer to maintain protein sulfhydryls in reduced form (34). Tubulin cysteine-SH groups in the reduced form are essential for microtubules to maintain their polymerization state (35). Recent studies showed that microcystins could conjugate with GSH and cysteine in both cell-free systems and in rat liver (23-25). Therefore, it is possible that microcystin may disrupt the cytoskeletal structure by directly binding with the tubulin cysteine residues after it enters the cells. Environmental carcinogens such as cadmium and arsenite have a high affinity to GSH and also to affect the cytoskeletal organization by blocking certain tubulin-SH groups (22). Tubulin synthesis is controlled by a unique autoregulatory feedback in which the pool of free (depolymerized) tubulin monomers regulates the level of new tubulin synthesis by modulating the stability of tubulin mRNA (36). The initial reaction of MCE-induced depolymerization depolymerization /de·po·lym·er·iza·tion/ (de?po-lim?er-i-za´shun) the conversion of a polymer into its component monomers. depolymerization of MTs may increase the level of free tubulin and thus trigger the feedback inhibition of new tubulin synthesis. This would further impair the formation of intact microtubules and may in part explain the severe loss of MTs in MCE-treated cells even though the intracellular GSH level was significantly increased. However, the increased GSH level may favor the assembly of MTs and maintain its stability. This important role of GSH has been further demonstrated in our present study: NAC could significantly alleviate MCE-induced MT and MF changes. GSH is the major cellular nonprotein thiol thiol: see mercaptan. reductant reductant /re·duc·tant/ (re-duk´tant) the electron donor in an oxidation-reduction (redox) reaction. re·duc·tant n. A reducing agent. and participates in numerous cellular processes such as intermediary metabolism and protection of cells against oxidative stress (37). In the present study, exposure to MCE for 6 hr showed a dose-dependent increase of intracellular GSH. However, the time-course study surprisingly revealed a biphasic response, i.e., a steady increase of GSH after 3 hr treatment and attainment of the highest concentration at approximately 6 hr, followed by a decrease after 12 hr. This biphasic cellular GSH response is not unique. Similar alterations have been reported when cells were exposed to cadmium and arsenite (21). The depletion of intracellular GSH when cells were treated with MCE for 24 hr is probably due to the toxic effect of MCE as a result of cell membrane damage that leads to cell lysis and GSH efflux efflux Medtalk That which flows outward . The disruption of hepatocyte cytoskeleton by MCE probably plays a crucial role in its hepatotoxicty. MTs and MFs change after 1 hr exposure to MCE, whereas significant LDH leakage only occurred after 3 hr treatment. The initial MCE-GSH binding may trigger the synthesis of GSH, probably by activating [Gamma]-glutamylcysteine synthetase synthetase /syn·the·tase/ (-the-tas) a term used in the names of some of the ligases, no longer favored because of its similarity to synthase and its emphasis on reaction products. syn·the·tase n. , the rate-limiting enzyme for GSH biosynthesis Biosynthesis The synthesis of more complex molecules from simpler ones in cells by a series of reactions mediated by enzymes. The overall economy and survival of the cell is governed by the interplay between the energy gained from the breakdown of compounds (37). The finding that BSO, an inhibitor of [Gamma]-glutamylcysteine synthetase, diminishes the MCE-induced increase of cellular GSH suggests that new GSH is being synthesized to overcome the low level of intracellular GSH. The increase of intracellular GSH is probably a cellular response to protect from the toxic effect induced by MCE. This hypothesis is further supported by the evidence that when cells were pretreated with NAC, MCE-induced cytotoxicity as well as cytoskeleton changes were significantly reduced. In conclusion, we showed that MCE disrupted the cellular cytoskeleton and affected the homeostasis homeostasis Any self-regulating process by which a biological or mechanical system maintains stability while adjusting to changing conditions. Systems in dynamic equilibrium reach a balance in which internal change continuously compensates for external change in a feedback of cellular thiols in hepatocytes. These two changes could be the main cytotoxic effect of MCE. The increase of intracellular GSH soon after MCE treatment may protect the hepatotoxicity induced by MCE. However, whether MCE also induces phosphorylation of MAPS and consequently destabilizes MTs and/or is a secondary effect to IF changes remains to be determined. REFERENCES AND NOTES (1.) Carmichael WW. The toxins of cyanobacteria. Sci Am 270:78-86 (1994). (2.) Honkanen RE, Zwiller J, Moore RE, Daily SL, Khatra BS, Dukelow M, Boynton AL. Characterization of microcystin-LR, a potent inhibitor of type 1 and 2A protein phosphatase. J Biol Chem 265:19401-19404 (1990). (3.) Ressom R, Soong FS, Fitzgerald J, Turczynowicz L, Elsaadi O, Roder D, Maynard T, Falconer IR. Health Effects of Toxic Cyanobacteria (Blue-Green Algae). 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(33.) van Gorp RM, Broers JL, Reutelingsperger CP, Bronnenberg NM, Hornstra G, van Dam-Mieras MC, Heemskerk JW. Peroxide-induced membrane blebbing in endothelial cells associated with glutathione oxidation but not apoptosis. Am J Physiol 277:C20-28 (1999). (34.) Monte D, Ross D, Bellomo G, Eklow L, Orrenius L. Iterations in intracellular thiol homeostasis during the metabolism of menadione menadione /men·a·di·one/ (men?ah-di´on) vitamin K3. 1. a synthetic fat-soluble vitamin that can be converted in the body to active vitamin K. 2. by isolated rat hepatocytes. Arch Biochem Biophys 235:334-342 (1984) (35.) Mellon M, Rebhum LI. Studies on the accessible sulfhydryls of polymerizable tubulin. In: Cell Motility. New York:Cold Spring Harbor Laboratory  The Cold Spring Harbor Laboratory , 1976;1146-1164. (36.) Ben-Ze'ev A, Farmer SR, Penman S. Mechanisms of regulating tubulin synthesis in cultured mammalian cells. Cell 17:319-325 (1979). (37.) Meister A. New aspects of glutathione biochemistry and transport: selective alteration of glutathione metabolism. Fed Proc 43:3031-3032 (1984). Wen-Xing Ding, Han-Ming Shen, and Choon-Nam Ong Center for Environmetal and Occupational Health, Department of Community, Ocuupational and Family Medicine, National University of Singapore The National University of Singapore (Abbreviation: NUS) is Singapore's oldest university. It is the largest university in the country in terms of student enrollment and curriculum offered. , Singapore Address correspondence to C.N. Ong, Center for Environmental and Occupational Health, Department of Community, Occupational and Family Medicine, MD3, National University of Singapore, Singapore 117597, Singapore. Telephone: 65 8744982. Fax: 65 7791489. E-mail: cofongcn@nus.edu.sg We thank E. Cornie and X. Wen for technical assistance in the confocal microscopy. W-X. Ding is supported by a research scholarship from National University of Singapore. Received 23 December 1999; accepted 1 February 2000. |
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