1 Vrije Universiteit Brussel, Laboratorium voor Cellulaire Genetica, Pleinlaan 2, 1050 Brussel, 2 Katholieke Universiteit Leuven, Laboratorium voor Pneumologie, Eenheid Longtoxicologie, Herestraat 49, B-3000 Leuven and 3 Université catholique de Louvain, Unité de Toxicologie industrielle et Médecine du Travail, Clos Chapelle aux Champs 30.54, B-1200 Bruxelles, Belgium
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Abstract |
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Abbreviations: AT-II, rat type II pneumocytes; BAL, broncho-alveolar lavage; i.t., intra-tracheal; PBMC, peripheral blood mononucleated cells; WC-Co, hard metal or cemented carbide
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Introduction |
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Lasfargues et al. (2,3) demonstrated that in vivo, in the rat, a WC-Co mixture containing 6% of Co (5.016.67 mg/kg body wt) caused acute and delayed pulmonary toxicity, leading to a pulmonary fibrosis reaction. In vitro, in human lymphocytes, the WC-Co mixture was genotoxic as evaluated with the alkaline comet and elution assays (DNA breaks and alkali-labile sites) and with the in vitro cytokinesis-block micronucleus test (chromosome/genome mutations) (46). One of the possible mechanisms underlying the genotoxicity of hard metal dust is a specific physicochemical interaction between Co metal and WC particles, which leads to an excessive formation of active oxygen species (7), probably peroxides (8). No experimental data are available on the in vivo mutagenic and carcinogenic potential of hard metal dust in the target tissue, the lung (for review see ref. 9).
In a human biomonitoring study conducted in workers exposed to WC-Co particles, no significant genotoxic effects were detected in peripheral blood mononucleated cells (PBMC) (10). A limitation of the study was, however, that PBMC were used as reporter cells for possible genotoxic damage induced by dust inhalation.
Analogous to the in vivo gut micronucleus test for the evaluation of exposure to chemicals following the oral route (11), examining mutagenicity in lung cells in vivo appears very relevant for the evaluation of the carcinogenic potential of inhaled particles, especially in type II pneumocytes as they are the stem cells of the alveolar epithelium. Therefore, the main objective of the present study was to evaluate the in vivo genotoxicity of the WC-Co particle mixture in rat type II pneumocytes (AT-II). This was achieved by evaluation of DNA breaks and alkali-labile sites (alkaline comet assay) and of chromosome/genome mutations (micronucleus test) after a single intra-tracheal (i.t.) instillation. Animals treated with bleomycin were included as positive controls. In parallel, the alkaline comet assay was performed on cells obtained after broncho-alveolar lavage (BAL) and on PBMC.
This study provides the first proof of the in vivo mutagenic potential of hard metal dust since WC-Co particles induced micronuclei in type II pneumocytes of the rat after a single i.t. instillation. In PBMC of WC-Co-treated animals, no increase in DNA damage and micronuclei was observed.
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Materials and methods |
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The WC-Co consisted of 6.3% cobalt, 84% tungsten and 5.4% carbon (median particle size 2 µm). The particles were sterilized during 4 h, at 200°C. The applied doses are always expressed as WC-Co per kg body weight (e.g. 16.6 mg WC-Co/kg body wt corresponding to 1.0 mg Co/kg body wt).
Animals
Wistar male rats of 200 g were obtained from Elevage Janvier (Bagneux, France) and housed in plastic cages with wood dust bedding under controlled lighting conditions (12 h light/12 h dark). The rats were allowed free access to standard laboratory diet (Trouw Nutrition, Gent, Belgium) and tap water.
Preliminary study
A preliminary experiment was conducted to select the appropriate dose of WC-Co, which would cause minimum pulmonary damage. Based on this study, 16.6 mg WC-Co/kg body wt was chosen, because it induced up to 72 h post-instillation significant but relatively limited pulmonary toxicity as assessed by lung weight changes and cellular and biochemical (LDH, proteins) alterations in BAL fluid (Table I).
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Bleomycin (1.0 U/kg body wt) was dissolved in sterile de-ionized water and administered to the rats in the same way as WC-Co. Groups of animals receiving vehicle (sterile de-ionized water) were also included.
Determination of cobalt content
Cobalt was measured in blood, lung homogenates and BAL fluid by atomic absorption spectrometry (Varian Zeeman SpectrAA-30 equipped with a graphite furnace atomizer). Blood and homogenates were mineralized in concentrated nitric acid before analysis (12).
Pulmonary toxicity
A first set of animals (n = 30 in total) was killed with an overdose of nembutal (90 mg/kg, i.p.) at 12, 24, 48 or 72 h after i.t. dosing. The abdomen was opened and the abdominal aorta was cut to exsanguinate the animal. After opening the thorax, the left bronchus and pulmonary vessels were clamped and the left lung was removed, weighed (wet lung weight) and placed in an oven at 60°C for 48 h. Dry lung weight was obtained after the tissue had equilibrated to room temperature. Wet and dry lung weights are expressed relatively to body weight (mg/kg body wt).
The right lung was lavaged in situ four times with 4 ml 0.9% NaCl at room temperature via a 14 gauge Insyte-W catheter inserted into the trachea through a cut in the cricoid membrane. After recovery, the pooled BAL fluid was kept on ice until centrifugation at 250 g for 10 min at 4°C. The supernatant was assayed for total protein concentration and the activity of LDH with the Bio-Rad micro-assay procedure (Bio-Rad Laboratories N.V., Nazareth, Belgium). The pellet was resuspended in 200 µl PBS. One aliquot of the BAL cell suspension was used to calculate total cell count. Aliquots containing approximately 30 000 cells were diluted in 0.5 ml PBS and placed in the sample chamber of a Cytospin-3 cell centrifuge (Shandon Scientific, Cheshire, UK). Slides were stained using the Dade Diff-Quik (Baxter Diagnostics AG, Düdingen, Switzerland) staining set for differential cell counting (200 cells per animal were differentially counted).
Lung histology
After lavage, the right lung was instilled, using a syringe, with 6% formaldehyde in PBS until full expansion of the different lobes. Slices from all lung lobes were embedded in paraffin, 5 µm sections were prepared, stained with haematoxylineosin and examined by light microscopy by an experienced pathologist, who evaluated lung injury blindly. Observations were done in a semi-quantitative way, using a score from -, normal lung tissue; +, slight changes; ++, moderate and +++, severe change or damage.
Sampling and type II pneumocyte isolation
Another group of animals (n = 56 in total) was anaesthetized (pentobarbital 90 mg/kg i.p.), blood was taken by venipuncture of the vena cava with a pre-heparinized syringe to be used in the comet assay and for isolation of PBMC for the micronucleus test and then the rats were killed by exsanguination. After opening of the chest, the trachea was cannulated and the lungs were perfused in situ with 0.9% NaCl via the pulmonary artery.
BAL was performed by filling and emptying the lungs four times with 10 ml 0.9% NaCl. The BAL fluid was centrifuged, the total cell count was determined and the cells were processed in the alkaline comet assay.
AT-II cells were isolated following the procedure of Richards et al. (13) and as described previously in ref. 14. The lungs were trypsinised (250 mg/lung) at 37°C during 30 min and the enzyme activity was arrested by addition of 5 ml FCS. The digested tissue was then minced with scissors in the presence of DNase, shaken and filtered to obtain individual and/or clumps of a few cells. Further purification was achieved by centrifugation onto a discontinuous Percoll gradient (20 min, 300 g). The cells of the layer above the heavy gradient were plated in a Petri dish and incubated for 1 h at 37°C allowing fibroblasts and remaining macrophages to attach. The viability of the finally purified AT-II was assessed using the Trypan blue exclusion technique. The cells were resuspended in DMEM supplemented with 10% FCS, 1% penicillin/streptomycin, 0.5% fungizone and 1% glutamine and used immediately in the alkaline comet assay or plated onto chamber slides (16 well glass slides, Nalgen Nunc, IL) (300,000 cells/cm2). This procedure yielded an average purity of 90% AT-II cells (14).
Peripheral blood mononucleated cells isolation
After 1:1 dilution with PBS, the blood was layered onto Ficoll Paque. After 40 min centrifugation at 400 g, PBMC were isolated and washed with PBS (10 min centrifugation at 400 g). For the micronucleus test, the cells were cultured in RPMI 1640 medium supplemented with 10% fetal clone II, 2% PHA, 1% L-glutamine and 1% penicillin/streptomycin (triplicate 1 ml aliquots kept at 37°C). Cytochalasin B (6 µg/ml) was added 44 h after the start of the culture in order to block cytokinesis. After a total of 72 h culturing the PBMC were used in the cytokinesis-block micronucleus test (see below).
Alkaline comet assay with internal standard
The alkaline comet assay was performed on freshly isolated AT-II, BAL cells and whole blood. An appropriate amount of cells was mixed with 300 µl of low melting point agarose (0.8% w/v in PBS) and loaded onto a regular pre-coated microscopic slide (normal melting point agarose, 1% w/v in water). The comet assay was performed as described previously (6) including internal standards of untreated and ethylmethane sulfonate exposed K562 cells according to De Boeck et al. (15). Briefly, after lysis at 4°C (2.5 M NaCl, 100 mM Na2EDTA, 10 mM Tris, supplemented with 1% Triton X-100 and 10% DMSO just before use), unwinding of the DNA was performed in a buffer containing 300 mM NaOH, 1 mM Na2EDTA (pH >13, 17°C) during 40 min. Alkaline electrophoresis was performed in the same buffer for 20 min at 0.7 V/cm (25 V, 300 mA). The slides were then washed three times for 5 min each with neutralization buffer (0.4 M Tris, pH 7.5) and dehydrated in 100% ice-cold ethanol (10 min). To visualize and analyse the DNA damage, the slides were rehydrated with deionized water (200 µl, 10 min) and stained with ethidium bromide (20 µg/ml, 10 min). Fifty randomly chosen, non- overlapping, comets per coded duplicate slide (100 cells/animal) were captured using a Leitz fluorescence microscope (25x objective) coupled to a CCD camera and an image analysis system (Komet 3.0, Kinetic Imaging, Liverpool, UK). All slides were scored by a single person. Percentage of DNA in the tail (TD) was recorded as DNA migration parameter. Data are presented as corrected TD values, i.e. recalculated by applying the formula presented in (15), in which the median TD for a given animal/cell type (100 comets) is divided by the median TD of the concurrent negative internal standard.
Micronucleus test
The frequency of micronuclei was assessed in isolated type II pneumocytes (ex vivo) and in PBMC (ex vivo/in vitro, cytokinesis-block method).
Type II pneumocytes were fixed with 100% methanol (20 min) after 2 days of culture and stained with acridine orange (0.012% in phosphate buffer) prior to analysis with a Zeiss Axioscop fluorescence microscope (magnification 400x). Multiple culture wells on different coded chamber slides were analysed for each animal. In total, 2000 AT-II cells per animal were evaluated for the presence of micronuclei.
PBMC were cytospinned onto microscope slides and fixed with 100% methanol (20 min). The cells were stained with 5% Giemsa in Sörensen buffer (pH 6.8). Slides from triplicate cultures were analysed for each treatment point. Cytokinesis-blocked (binucleated) lymphocytes were examined for the presence of micronuclei (10003000 cells/animal). All coded slides were analysed with a Zeiss light microscope (1250x magnification).
The microscopical analysis of the micronucleus test was performed by a single person.
Statistical analysis
For pulmonary toxicity, differences between vehicle-treated animals and WC-Co or bleomycin-treated animals were evaluated using one-way ANOVA followed when appropriate by a Dunnett multiple comparison test. For genotoxicity, pairwise differences between pooled vehicle-treated animals and WC-Co or bleomycin-treated animals were assessed using the Student's t-test and the MannWhitney U test for the micronucleus test and comet assay, respectively.
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Results |
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Induction of DNA migration in AT-II, BAL cells and PBMC: alkaline comet assay
Figure 4ac presents the results of the alkaline comet assay (relative tail DNA) performed on AT-II, BAL cells and PBMC of rats at different time points after i.t. instillation of WC-Co (16.6 mg WC-Co/kg body wt) or bleomycin (1.0 U/kg body wt). The dotted line indicates the average DNA migration in vehicle-treated animals (n = 8; AT-II: 1.22 ± 0.51, BAL cells: 13.23 ± 3.69, PBMC: 0.61 ± 0.28).
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In BAL cells of vehicle-treated rats, the first observation was a higher level of DNA migration as compared with AT-II and PBMC (dotted line); the DNA migration levels were similar to those of untreated animals (data not shown). BAL cells of WC-Co and bleomycin-treated animals showed statistically significantly lower levels of DNA migration as compared with the vehicle controls.
In PBMC, no statistically significant difference in the level of DNA migration between WC-Co or bleomycin-treated and vehicle-treated animals was observed.
Induction of micronuclei in type II pneumocytes
Figure 5 displays the frequencies of micronucleated type II pneumocytes in a time course experiment in which rats underwent i.t. instillation with WC-Co (16.6 mg WC-Co/kg body wt) or bleomycin (1.0 U/kg body wt). The dotted line indicates the average frequency of micronucleated AT-II in vehicle-treated animals ( MN AT-II: 2.4 ± 2.3; n = 9).
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Based on these data, only the 72 h time point was chosen to perform a dose-effect study. Table II presents the frequencies of micronucleated AT-II in rats exposed intra-tracheally to four doses of WC-Co (1.8, 5.5, 16.6 and 49.8 mg WC-Co/kg body wt), bleomycin (1.0 U/kg body wt) or vehicle (water). The second highest dose of WC-Co (16.6 mg WC-Co/kg body wt) was the only one to cause a statistically significant increase in the frequency of micronucleated AT-II. Treatment with the other doses led to a small but non-significant increase of MN as compared with the vehicle-treated rats. Bleomycin induced a statistically significant increase in the frequency of micronucleated AT-II as compared with the vehicle-treated animals.
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Discussion |
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This study provides the first proof of the in vivo mutagenicity of hard metal dust in a target cell type, i.e. type II pneumocytes in the rat. Seventy-two hours after i.t. instillation of a subtoxic dose of WC-Co, a statistically significant increase in micronucleated AT-II was found. This observation was preceded by an increase in DNA damage detected with the alkaline comet assay in AT-II at 12 h after exposure. In BAL cells, the alkaline comet assay showed decreased DNA migration in exposed animals and, in PBMC, no significant differences could be detected in animals treated with WC-Co both with the alkaline comet assay or the cytokinesis-block micronucleus test.
Particles, together with fibres, form a rather specific group of toxic agents. Genotoxicity by inhalation of particles is believed to follow two predominant pathways (20,21): (i) active oxygen species, produced because of specific surface properties or the presence of transition metals, together with other parameters such as particle size, shape and uptake, play a major role in the primary genotoxicity of particles; (ii) secondary genotoxicity, mediated by the excessive and persistent formation of active oxygen species by inflammatory cells, combined with increased proliferation of type II pneumocytes, may act to initiate and promote genotoxic effects in lung epithelial cells after chronic exposure to toxic particles. Either or both mechanisms are likely to be at play in the case of WC-Co particles as they were demonstrated to cause excessive formation of active oxygen species (7) and pulmonary inflammation (2,3). In addition, WC-Co was found to inhibit DNA repair, to interact with the mitotic spindle inducing chromosome loss, and to cause less apoptosis than its single components in vitro in human PBMC (22).
The observation in the present study of the highest increase in micronucleated AT-II at 72 h after i.t. instillation of WC-Co, is not unexpected because it parallels the time required for these cells to complete one division (23). The nature of the micronuclei induced in the AT-II is not clear at this point, i.e. whether they originate from a whole chromosome (aneugenic event) or from an acentric fragment (clastogenic event). Given the presence of intruding inflammatory cells, one cannot exclude that the mutagenic events detected in the AT-II are, besides being due to genotoxicity of the WC-Co particles, the result of inflammation (secondary genotoxicity as suggested in ref. 21). Indeed, already at 12 h post-instillation of WC-Co a substantial increase in inflammatory cells was observed. Their presence in the alveoli before and during the proliferation of the AT-II could contribute to the formation of the observed micronuclei. The sporadic presence of cells other than AT-II on the chamber slides did not hamper the microscopical analysis because AT-II could easily be distinguished due to their specific cytoplasmic and nuclear characteristics.
The fact that, at 72 h, the highest dose of WC-Co (49.8 mg/kg) induced a lower frequency of micronucleated AT-II than the second highest tested dose (16.6 mg WC-Co/kg body wt) possibly indicated that this 3-fold higher dose caused either mitotic delay or cell death. It should, however, be kept in mind that for most time points other than 72 h, results from only a limited number of animals were available and they should therefore not be considered as conclusive. At later time points, the number of micronucleated type II pneumocytes after WC-Co treatment (16.6 mg WC-Co/kg body wt) decreased, while this frequency remained higher in the bleomycin exposed rats. This difference might be related to the fact that cobalt was rapidly removed from the lungs and that, at that time point, a lower frequency of inflammatory cells was present in the alveoli, both factors contributing to reduce the burst of active oxygen species released in the alveoli. Another possibility is the occurrence of cell death and/or mitotic delay at later time points after WC-Co treatment.
The observation of a statistically significant increase in DNA migration in AT-II at 12 h (and the return to baseline afterwards) after instillation of WC-Co, could be related to the presence of inflammatory cells exerting oxidative stress. The non-significant increase observed for bleomycin could, however, suggest that, for this endpoint, earlier sampling times (immediately after instillation) would be required to detect a significant effect. This would be in line with the idea that the alkaline comet assay detects transiently occurring DNA strand breaks and alkali labile sites. However, it should be kept in mind that the isolation of the AT-II itself requires at least 6 h, a period during which DNA strand break repair could take place.
The decrease in DNA migration observed in BAL cells of WC-Co- and bleomycin-treated rats is probably related to changes in the relative proportion of exposed (resident macrophages) and non-exposed cells (recruited inflammatory cells consisting of lymphocytes, neutrophils and eosinophils) as indicated by the differential cell counts of the BAL cell population. Unfortunately, and in contrast to the microscopical analysis of AT-II for the micronucleus test, no distinction could be made between the macrophages and the other cell types on the basis of comet appearance of the BAL cells.
In PBMC, no significant difference could be detected in animals treated with WC-Co both with the alkaline comet assay or the ex vivo/in vitro cytokinesis-block micronucleus test at any of the considered time points. The observation of a small but not statistically significant increase in micronucleated binucleated cells 72 h after bleomycin exposure suggests a potential of PBMC as reporter cells for genotoxic damage induced in the lung, when the agent is, at least partially, systemically distributed. This is not the case for a particulate agent such as the WC-Co mixture. Therefore, there is a need to re-evaluate cautiously the relevance of PBMC as reporter cells to assess lung effects induced by inhaled particulate agents. In order to draw firm conclusions, other relevant positive controls should be tested and further confirmation with regard to biomonitoring strategies is required.
In summary, this study introduced the use of isolated type II pneumocytes for the assessment of in vivo genotoxicity. WC-Co particles are able to induce micronuclei in type II pneumocytes of the rat after i.t. instillation. Further characterization of micronuclei with pan-centromeric probes to distinguish between the induction of chromosome and genome mutations would provide valuable mechanistic information. Parallel decreased DNA migration in BAL cells reflected change in BAL cell populations, accompanying the inflammatory response. No corresponding change in micronucleus frequencies could be detected in PBMC. Induction of apoptosis is another endpoint that should be taken into account, as it may specifically eliminate mutated cells. It could also be considered to look at more relevant target cell types for lung cancer (e.g. bronchial epithelial cells) and the specific involvement of inflammatory cells in genotoxic effects.
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Notes |
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* Both authors contributed equally to this work.
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Acknowledgments |
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References |
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