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3. Re-evaluation of chromosomal aberration induction on nine mouse lymphoma assay ‘unique positive’ NTP carcinogens

Author

Matsuoka, A., primary, Yamakage, K., additional, Kusakabe, H., additional, Wakuri, S., additional, Asakura, M., additional, Noguchi, T., additional, Sugiyama, T., additional, Shimada, H., additional, Nakayama, S., additional, Kasahara, Y., additional, Takahashi, Y., additional, Miura, K.F., additional, Hatanaka, M., additional, Ishidate, M., additional, Morita, T., additional, Watanabe, K., additional, Hara, M., additional, Odawara, K., additional, Tanaka, N., additional, Hayashi, M., additional, and Sofuni, T., additional

Published
1996
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11. An international validation study of the IL-2 Luc assay for evaluating the potential immunotoxic effects of chemicals on T cells and a proposal for reference data for immunotoxic chemicals.

Author

Kimura Y, Yasuno R, Watanabe M, Kobayashi M, Iwaki T, Fujimura C, Ohmiya Y, Yamakage K, Nakajima Y, Kobayashi M, Mashimo N, Takagi Y, Omori T, Corsini E, Germolec D, Inoue T, Rogen EL, Kojima H, and Aiba S

Subjects
Cell Line, Cell Proliferation drug effects, Humans, Interleukin-2 genetics, Luciferases metabolism, Reproducibility of Results, T-Lymphocytes immunology, Biological Assay, Immunologic Factors toxicity, Interleukin-2 immunology, T-Lymphocytes drug effects, Toxicity Tests methods
Abstract

To evaluate the immunotoxic effects of xenobiotics, we have established the Multi-ImmunoTox assay, in which three stable reporter cell lines are used to evaluate the effects of chemicals on the IL-2, IFN-γ, IL-1β and IL-8 promoters. Here, we report the official validation study of the IL-2 luciferase assay (IL-2 Luc assay). In the Phase I study that evaluated five coded chemicals in three sets of experiments, the average within-laboratory reproducibility was 86.7%. In the Phase II study, 20 coded chemicals were evaluated at multiple laboratories. In the combined results of the Phase I and II studies, the between-laboratory reproducibility was 80.0%. These results suggested that the IL-2 Luc assay was reproducible both between and within laboratories. To determine the predictivity, we collected immunotoxicological information and constructed the reference data by classifying the chemical into immunotoxic compounds targeting T cells or others according to previously reported criteria. When compared with the reference data, the average predictivity of the Phase I and II studies was 75.0%, while that of additional 60 chemicals examined by the lead laboratory was 82.5%. Although the IL-2 Luc assay alone is not sufficient to predict immunotoxicity, it will be a useful tool when combined with other immune tests., Competing Interests: Declaration of Competing Interest The authors declare that they have no known competing financial interests or personal relationships that could have appeared to influence the work reported in this paper., (Copyright © 2020 The Authors. Published by Elsevier Ltd.. All rights reserved.)

Published
2020
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12. Collaborative study of thresholds for mutagens: proposal of a typical protocol for detection of hormetic responses in cytotoxicity tests.

Author

Sutou S, Koeda A, Komatsu K, Shiragiku T, Seki H, Yamakage K, Niitsuma T, Kudo T, and Wakata A

Abstract

Background: According to the linear no-threshold model (LNT), even the smallest amount of radiation is hazardous. Although the LNT is not based on solid data, this hypothesis has been applied to mutagens and carcinogens. As a result, it has been postulated that there are no thresholds for these chemicals. To demonstrate negativity by experiments is practically impossible, because negative data may leave behind the possibility that additional data might make the resolution power high enough to change negativity to positivity. Furthermore, additional data collection may be endless and we may be trapped in agnosticism. When hormesis is established, in which biological responses are higher at low-doses and lower at high-doses than the control, thresholds could be established between the low- and high-doses. Before examination of thresholds in chemical mutagenesis, hormetic responses in cytotoxicity were tested using cultured mammalian cells., Method: Human cells (HeLa S3 and TK6) or Chinese hamster cells (CHL/IU) were cultured in 96-well plates and treated with mitomycin C (MMC) or ethyl methanesulfonate (EMS) at various dose levels and optical density was measured after addition of a reagent to detect cellular activity. In hormetic responses, data might fluctuate to and fro; therefore, experimental conditions were examined from various aspects to eliminate confounding factors including cell numbers, detection time, the edge effect of 96-well plates, and measurement time after addition of the reagent for detection., Results: The dose response relationship was never linear. Cellular activities after treatment with MMC or EMS were generally higher at lower doses levels and lower at higher doses than the control, showing hormesis and allowing the establishment of thresholds. Dose response curves sometimes showed two or three peaks, probably reflecting different cellular responses., Conclusion: Hormetic responses in cytotoxicity tests were observed and thresholds could be established. Based on the results of this investigation, we put forward a tentative protocol to detect chemical hormesis in cytotoxicity tests, i.e., inoculate 2000 cells per well, add various doses of a test chemical 48 h after inoculation, add a detection dye 10 h after treatment, and measure optical density 2 h after addition of the reagent for detection., Competing Interests: Not applicable.Not applicable.The authors declare that they have no competing interests.Springer Nature remains neutral with regard to jurisdictional claims in published maps and institutional affiliations.

Published
2018
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13. The performance of an in vitro skin sensitisation test, IL-8 Luc assay (OECD442E), and the integrated approach with direct peptide reactive assay (DPRA).

Author

Kimura Y, Watanabe M, Suzuki N, Iwaki T, Yamakage K, Saito K, Nakajima Y, Fujimura C, Ohmiya Y, Omori T, Kojima H, and Aiba S

Subjects
Biological Assay, Genes, Reporter, Glyceraldehyde-3-Phosphate Dehydrogenases genetics, Humans, Interleukin-8 genetics, Luciferases genetics, Peptides, THP-1 Cells, Animal Testing Alternatives, Dermatitis, Allergic Contact, Haptens toxicity, Skin Tests
Abstract

In all current in vitro skin sensitisation assays, DMSO is used to dissolve water-insoluble chemicals. However, our previous study suggested the superiority of the modified IL-8 Luc assay (mIL-8 Luc), in which X-VIVO TM 15 is used to dissolve chemicals, over the original assay using DMSO (oIL-8 Luc). In this study, to confirm the superiority of the mIL-8 Luc, we first increased the number of chemicals examined and demonstrated the superiority of the mIL-8 Luc, in which the mIL-8 Luc provided 87.6% of sensitivity, 74.2% of specificity, and 84.6% of accuracy. Next, to clarify the cause of false negative judgment by the mIL-8 Luc, we examined the effects of physical properties of chemicals on judgment. The results demonstrated that high molecular weight, high LogKo/w, or poor water solubility, did not cause false negative judgment. When it was accepted as an OECD test guideline, the criteria of the mIL-8 Luc to determine sensitisers were modified to further decrease false negative judgment by poor solubility. By applying the new criteria, the test guideline IL-8 Luc assay (tgIL-8 Luc) improved sensitivity but decreased specificity and increased the number of chemicals that cannot be judged. To overcome this problem, we examined a simple combination of the tgIL-8 Luc with direct peptide reactive assay (DPRA), which could improve specificity and decrease the number of the chemicals that cannot be judged. These data suggest that the tgIL-8 Luc is a promising in vitro skin sensitisation assay in combination with other in vitro or in chemico methods.

Published
2018
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14. A Cytoplasmic Form of Gaussia luciferase Provides a Highly Sensitive Test for Cytotoxicity.

Author

Tsuji S, Ohbayashi T, Yamakage K, Oshimura M, and Tada M

Subjects
Adenosine Triphosphate metabolism, Animals, Antineoplastic Agents pharmacology, Carbon Tetrachloride pharmacology, Carcinoma, Hepatocellular drug therapy, Carcinoma, Hepatocellular metabolism, Genes, Reporter, Humans, Liver Neoplasms drug therapy, Liver Neoplasms metabolism, Liver Neoplasms pathology, Luciferases genetics, Luminescence, Reproducibility of Results, Tumor Cells, Cultured, Apoptosis drug effects, Biological Assay methods, Carcinoma, Hepatocellular pathology, Copepoda enzymology, Cytoplasm enzymology, Luciferases metabolism
Abstract

The elimination of unfavorable chemicals from our environment and commercial products requires a sensitive and high-throughput in vitro assay system for drug-induced hepatotoxicity. Some previous methods for evaluating hepatotoxicity measure the amounts of cytoplasmic enzymes secreted from damaged cells into the peripheral blood or culture medium. However, most of these enzymes are proteolytically digested in the extracellular milieu, dramatically reducing the sensitivity and reliability of such assays. Other methods measure the decrease in cell viability following exposure to a compound, but such endpoint assays are often confounded by proliferation of surviving cells that replace dead or damaged cells. In this study, with the goal of preventing false-negative diagnoses, we developed a sensitive luminometric cytotoxicity test using a stable form of luciferase. Specifically, we converted Gaussia luciferase (G-Luc) from an actively secreted form to a cytoplasmic form by adding an ER-retention signal composed of the four amino acids KDEL. The bioluminescent signal was >30-fold higher in transgenic HepG2 human hepatoblastoma cells expressing G-Luc+KDEL than in cells expressing wild-type G-Luc. Moreover, G-Luc+KDEL secreted from damaged cells was stable in culture medium after 24 hr at 37°C. We evaluated the accuracy of our cytotoxicity test by subjecting identical samples obtained from chemically treated transgenic HepG2 cells to the G-Luc+KDEL assay and luminometric analyses based on secretion of endogenous adenylate kinase or cellular ATP level. Time-dependent accumulation of G-Luc+KDEL in the medium increased the sensitivity of our assay above those of existing tests. Our findings demonstrate that strong and stable luminescence of G-Luc+KDEL in human hepatocyte-like cells, which have high levels of metabolic activity, make it suitable for use in a high-throughput screening system for monitoring time-dependent cytotoxicity in a limited number of cells.

Published
2016
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15. In vivo comet assay of acrylonitrile, 9-aminoacridine hydrochloride monohydrate and ethanol in rats.

Author

Nakagawa Y, Toyoizumi T, Sui H, Ohta R, Kumagai F, Usumi K, Saito Y, and Yamakage K

Subjects
Animals, Carcinogens toxicity, DNA Damage drug effects, Dose-Response Relationship, Drug, Liver drug effects, Male, Rats, Rats, Sprague-Dawley, Stomach drug effects, Acrylonitrile toxicity, Aminacrine toxicity, Comet Assay methods, Ethanol toxicity
Abstract

As part of the Japanese Center for the Validation of Alternative Methods (JaCVAM)-initiative international validation study of the in vivo rat alkaline comet assay, we examined the ability of acrylonitrile, 9-aminoacridine hydrochloride monohydrate (9-AA), and ethanol to induce DNA damage in the liver and glandular stomach of male rats. Acrylonitrile is a genotoxic carcinogen, 9-AA is a genotoxic non-carcinogen, and ethanol is a non-genotoxic carcinogen. Positive results were obtained in the liver cells of male rats treated with known genotoxic compounds, acrylonitrile and 9-AA., (Copyright © 2015 Elsevier B.V. All rights reserved.)

Published
2015
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16. Modifications of azoxymethane-induced carcinogenesis and 90-day oral toxicities of 2-tetradecylcyclobutanone as a radiolytic product of stearic acid in F344 rats.

Author

Sato M, Todoriki S, Takahashi T, Hafez E, Takasu C, Uehara H, Yamakage K, Kondo T, Matsumoto K, Furuta M, and Izumi K

Abstract

A 90-day oral toxicity test in rats was performed to evaluate the toxicity of 2-tetradecylcyclobutanone (2-tDCB), a unique radiolytic product of stearic acid. Six-week-old male and female F344 rats (n=15/group) were given 2-tDCB at concentrations of 0, 12, 60 and 300 ppm in a powder diet for 13 weeks. Slight dose-dependent increases in serum total protein and albumin in male rats were found, but these changes were not considered to be a toxic effect. The fasting, but not non-fasting, blood glucose levels of the male rats in the 300 ppm group and female rats in the 60 and 300 ppm groups were lower than those of the controls. Gas chromatography-mass spectrometry analysis showed dose-dependent accumulation of 2-tDCB in adipose tissue, notably in males. Next, we performed an azoxymethane (AOM)-induced two-stage carcinogenesis study. After injection of 6-week-old male F344 rats (n=30/group) once a week for 3 weeks, the animals received 2-tDCB at concentrations of 0, 10, 50 and 250 ppm in a powder diet for 25 weeks. The incidences of colon tumors for the 2-tDCB dosages were 34%, 45%, 40% and 37%, respectively, and were not statistically significant. These data suggest that 2-tDCB shows no toxic or tumor-modifying effects under the present conditions, and that the no-observed-adverse-effect level for 2-tDCB is 300 ppm in both sexes, equivalent to 15.5 mg/kg b.w./day in males and 16.5 mg/kg b.w./day in females.

Published
2015
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17. Genotoxic potential and in vitro tumour-promoting potential of 2-dodecylcyclobutanone and 2-tetradecylcyclobutanone, two radiolytic products of fatty acids.

Author

Yamakage K, Sui H, Ohta R, Toyoizumi T, Kawakami K, Matsumoto H, Takahashi T, Sasaki K, Ikezumi M, Negishi S, Izumi K, Todoriki S, Takashi K, and Furuta M

Subjects
Animals, Azoxymethane toxicity, Carcinogens toxicity, Cell Line, Chromosome Aberrations drug effects, Colon drug effects, Colon pathology, Comet Assay, Cricetinae, Dose-Response Relationship, Drug, Female, Food Irradiation, Male, Mice, Mice, Inbred ICR, Micronucleus Tests, Mutagenicity Tests, Mutagens toxicity, Neoplasms chemically induced, Rats, Rats, Sprague-Dawley, Salmonella typhimurium drug effects, Cyclobutanes toxicity, DNA Damage drug effects, Fatty Acids chemistry
Abstract

The DNA-damaging and tumour-promoting effects of two 2-alkylcyclobutanones (2-ACBs), which are found in irradiated fat-containing foods, were investigated by use of the comet assay and in an azoxymethane (AOM)-induced colon-carcinogenesis study in rats, respectively. We conducted genotoxicity tests of 2-dodecylcyclobutanone (2-dDCB) and 2-tetradecylcyclobutanone (2-tDCB) according to the test guidelines for chemicals or drugs. In addition, a cell-transformation assay with Bhas 42 cells was performed to investigate their promoting potential in vitro. The Salmonella typhimurium mutagenicity assay (Ames test), conducted with five tester strains, revealed that neither 2-dDCB nor 2-tDCB possessed mutagenic activity. Moreover, both in the in vitro chromosomal aberration test on CHL/IU cells and the in vivo bone-marrow micronucleus test where mice were given 2-dDCB and 2-tDCB (orally, up to 2000 mg/kg bw/day), we did not detect any clastogenic effects. Furthermore, DNA strand-breaks were not detected in the in vitro comet assay with CHL/IU cells, and DNA adducts derived from 2-dDCB and 2-tDCB were not detected in the colon tissues of the mice used for the micronucleus tests, in rats from a repeated dose 90-day oral toxicity test (0.03% 2-tDCB in the diet), or in rats from the AOM-induced carcinogenesis study (0.025% 2-tDCB in the diet). An in vitro tumour-promotion assay with Bhas 42 cells revealed that the number of transformed foci increased significantly following treatment of cells in the stationary phase with 2-dDCB or 2-tDCB for 10 days. Our results indicate that neither 2-dDCB nor 2-tDCB were genotoxic chemicals. However, they exhibited promoting activity, at least in vitro, when Bhas 42 cells were continuously exposed to these chemicals at toxic doses., (Copyright © 2014 Elsevier B.V. All rights reserved.)

Published
2014
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18. In vitro clastogenicity and phototoxicity of fullerene (C(60)) nanomaterials in mammalian cells.

Author

Honma M, Takahashi T, Asada S, Nakagawa Y, Ikeda A, and Yamakage K

Subjects
Animals, BALB 3T3 Cells, Cell Line, Cell Survival, Chromosome Aberrations, Cricetinae, Cricetulus, DNA Damage, Humans, Mice, Micronucleus Tests, Polyploidy, Dermatitis, Phototoxic, Fullerenes toxicity, Mutagens toxicity, Nanostructures toxicity
Abstract

Carbon nanomaterials such as carbon nanotubes, graphene, and fullerenes (C(60)) are widely used in industry. Because of human health concerns, their toxic potential has been examined in vivo and in vitro. Here we used mammalian cells to examine the in vitro clastogenicity as well as the phototoxicity of C(60). While C(60) induced no structural chromosome aberrations in CHL/IU cells at up to 5mg/ml (the maximum concentration tested), it significantly induced polyploidy at 2.5 and 5mg/ml with and without metabolic activation. In BALB 3T3 cells, C(60) showed no phototoxic potential but the anatase form of titanium oxide did. Since insoluble nanomaterials cause polyploidy by blocking cytokinesis rather than by damaging DNA, we concluded that the polyploidy induced by C(60) in CHL/IU cells was probably due to non-DNA interacting mechanisms., (Copyright © 2012 Elsevier B.V. All rights reserved.)

Published
2012
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19. Molecular mechanisms of apoptosis induction by 2-dodecylcyclobutanone, a radiolytic product of palmitic acid, in human lymphoma U937 cells.

Author

Yu DY, Zhao QL, Furuta M, Todoriki S, Izumi K, Yamakage K, Matsumoto K, Nomura T, and Kondo T

Subjects
Calcium metabolism, Cell Survival drug effects, Cytochromes c metabolism, Gene Expression Regulation drug effects, Humans, Mitochondria metabolism, Proto-Oncogene Proteins c-bcl-2 genetics, Proto-Oncogene Proteins c-bcl-2 metabolism, Reactive Oxygen Species metabolism, U937 Cells, bcl-2-Associated X Protein genetics, bcl-2-Associated X Protein metabolism, Apoptosis drug effects, Cyclobutanes toxicity, Food Irradiation adverse effects, Palmitic Acid chemistry
Abstract

The irradiation of fat-containing food forms 2-dodecylcyclobutanone (2-DCB) from palmitic acid (PA). In this study, we investigated whether 2-DCB and PA induce apoptosis in human lymphoma U937 cells. We found that cell viability decreased by 2-DCB and apoptosis was induced by 2-DCB and PA. 2-DCB and PA significantly enhanced the formation of intracellular reactive oxygen species (ROS). Apoptosis induced by 2-DCB and PA was strongly prevented by an antioxidant, N-acetyl-L: -cysteine. The treatment with 2-DCB and PA resulted in the loss of mitochondrial membrane potential, and Fas, caspase-8 and caspase-3 activation. Pretreatment with a pan-caspase inhibitor (z-VAD) significantly inhibited apoptosis induced by 2-DCB and PA. Moreover, 2-DCB and PA also induced Bax up-regulation, the reduction in Bcl-2 expression level, Bid cleavage and the release of cytochrome c from the mitochondria to the cytosol. In addition, an increase in intracellular Ca(2+) concentration ([Ca(2+)](i)) was observed after the treatment with 2-DCB and PA. Our results indicated that intracellular ROS generation, the modulation of the Fas-mitochondrion-caspase-dependent pathway and the increase in [Ca(2+)](i) involved in apoptosis are induced by 2-DCB and PA in U937 cells.

Published
2012
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20. Usefulness of combined in vivo skin comet assay and in vivo skin micronucleus test.

Author

Toyoizumi T, Ohta R, Kawakami K, Nakagawa Y, Tazura Y, Kuwagata M, Noguchi S, Sui H, and Yamakage K

Subjects
Animals, Comet Assay methods, Liver drug effects, Male, Mice, Mice, Nude, Micronucleus Tests methods, Carcinogens toxicity, Mutagens toxicity, Skin drug effects
Abstract

We have already found that the in vivo skin comet assay is useful for the evaluation of primary DNA damage induced by genotoxic chemicals in epidermal skin cells. The aim of the present study was to evaluate the sensitivity and specificity of the combined in vivo skin comet assay and in vivo skin micronucleus (MN) test using the same animal to explore the usefulness of the new test method. The combined alkaline comet assay and MN test was carried out with three chemicals: 4-nitroquinoline-1-oxide (4NQO), N-methyl-N'-nitro-N-nitrosoguanidine (MNNG) and benzo[a]pyrene (B[a]P). In the first experiment, we compared DNA- and chromosome-damaging effects of 3 [72, 24 and 3 hours (h) before sacrifice] and 4 applications (72, 48, 24 and 3h before sacrifice) of 4NQO, which induces dermal irritancy. The animals were euthanized and their skin was sampled for the combination test. As a result, the 4-application method was able to detect both DNA- and chromosome-damaging potential with a lower concentration; therefore, in the second experiment, MNNG and B[a]P were topically applied four times, respectively. The animals were euthanized, and then their skins were sampled for combination tests. In the alkaline comet assay, significant differences in the percent of DNA (%DNA) in the tail were observed in epidermal skin cells treated with MNNG and B[a]P. In the MN test, an increased frequency of MN cells (%MN) cells was observed by treatment with MNNG; however, there were no significant increases. In contrast, significant differences in %MN were observed by treatment with B[a]P. From these results, we conclude that the combined in vivo skin comet assay and in vivo MN test was useful because it can detect different genotoxicity with the same sampling time and reduce the number of animals used., (© 2012 Elsevier B.V. All rights reserved.)

Published
2012
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21. Evaluation of effect during cell isolation process in alkaline comet assay using epidermal skin cells.

Author

Toyoizumi T, Watanabe M, Sui H, Nakagawa Y, Ohta R, and Yamakage K

Subjects
Cells, Cultured, DNA Damage, Humans, Hydrogen-Ion Concentration, Trypsin, Cell Separation methods, Comet Assay, Edetic Acid toxicity, Epidermal Cells
Abstract

The aim of the present study was to evaluate the effect of the cell isolation process in the alkaline comet assay using epidermal skin cells. When we explored the cell isolation method for the alkaline comet assay using the 3-dimensional (3D) human epidermal skin model, we found that DNA damage and cytotoxicity were induced during the cell isolation process. In particular, trypsin 5 min treatment with ethylene diamine tetraacetic acid (EDTA) showed about 5 times %DNA in the tail value compared to without EDTA treatment. In general, EDTA is commonly used for cell isolation, but it is known to induce genotoxicity due to secondary effects. We therefore evaluated the effect of EDTA and pH in the alkaline comet assay on a monolayer culture of rat keratinocytes. As a result, there was a significant increase of %DNA in tail values by treatment with 0.1 w/v% EDTA for 60 min; however, there was no difference in the %DNA in tail values between 0.1 w/v% EDTA/PBS(-) (pH 6.8) and 0.1 w/v% EDTA/PBS(-) (pH 7.4). These data imply that there is a need to control the EDTA conditions for cell isolation in the epidermal skin cells.

Published
2012
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22. Use of the in vivo skin comet assay to evaluate the DNA-damaging potential of chemicals applied to the skin.

Author

Toyoizumi T, Ohta R, Nakagawa Y, Tazura Y, Kuwagata M, Noguchi S, and Yamakage K

Subjects
Animals, DNA Damage, Male, Mice, Mice, Hairless, Sensitivity and Specificity, Comet Assay methods, Mutagens toxicity, Skin drug effects
Abstract

The aim of the present study was to evaluate both sensitivity and specificity of an in vivo skin comet assay using chemically treated, hairless mouse dorsal skin as a model. N-methyl-N'-nitro-N-nitrosoguanidine (MNNG, 0.0125-0.2%), 4-nitroquinoline-1-oxide (4NQO, 0.01-0.25%), mitomycin C (MMC, 0.0125-0.05%), benzo[a]pyrene (B[a]P, 0.25-2%), and 7,12-dimethylbenz[a]anthracene (DMBA, 0.25-1%) were each applied once to the dorsal skin of hairless male mice; after 3h, epidermal skin cells were isolated, and the alkaline comet assay was performed. The assay was performed after 24h for only the B[a]P and DMBA. Furthermore, B[a]P and DMBA were evaluated by alkaline comet assay using liver cells after both 3 and 24h. The mean percent of DNA (%DNA) in tail in the 0.05-0.2% MNNG and 0.1-0.25% 4NQO treatment groups was markedly higher than in the control group at 3h post-application. Although the mean %DNA values in the tail in the B[a]P and DMBA groups were the same as the controls at 3h post-application, the 2% B[a]P and 1% DMBA groups showed significantly higher values versus controls 24h after application. No significant increases in the mean %DNA in the tail were observed in the MMC group. No clear increases in %DNA in the tail were observed in the B[a]P and DMBA groups at 3 or 24h after application in the liver. These results suggest that the in vivo skin comet assay is able to accurately identify DNA-damaging potential with a skin-specific response and is a useful method to detect the DNA-damaging potential of genotoxic chemicals on the skin., (Copyright © 2011 Elsevier B.V. All rights reserved.)

Published
2011
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23. SFTG international collaborative study on in vitro micronucleus test IV. Using CHL cells.

Author

Wakata A, Matsuoka A, Yamakage K, Yoshida J, Kubo K, Kobayashi K, Senjyu N, Itoh S, Miyajima H, Hamada S, Nishida S, Araki H, Yamamura E, Matsui A, Thybaud V, Lorenzon G, Marzin D, and Lorge E

Subjects
Aneugens toxicity, Animals, Bleomycin toxicity, Cell Line, Clofibrate toxicity, Colchicine toxicity, Cricetinae, Cytarabine toxicity, Cytochalasin B, Diethylstilbestrol toxicity, Fluorouracil toxicity, Griseofulvin toxicity, In Vitro Techniques, International Cooperation, Mannitol toxicity, Urethane toxicity, Micronucleus Tests methods, Mutagens toxicity
Abstract

In this report, are presented the results of an international collaborative study on the in vitro micronucleus assay, using CHL cells. Fourteen laboratories participated in this study which was coordinated by an organizing committee supported by the SFTG (the French branch of the European Environmental Mutagen Society). Nine coded substances, having different modes of action and at different levels were assessed in the in vitro micronucleus test, using a common protocol. Mitomycin C was used as a positive control. In order to help to define a standard protocol on CHL cells, short and long treatment periods followed by various recovery times, with or without cytochalasin B, were compared. After an evaluation of the acceptability of the assays, the tested chemicals were classified as negative, positive or equivocal. Mannitol and clofibrate were judged as negative in all treatment schedules. Bleomycin was positive in all the treatment schedules, with an increase in the number of micronucleated cells in both mononucleate and binucleate cells when using cytochalasin B. This was also shown for the aneugens colchicine, diethylstilboestrol and griseofulvin, as expected. Urethane was judged as equivocal only after long treatment with cytochalasin B, and negative in all other treatment schedules. In any case, no genotoxic compound would have been missed with schedules including a short and a long treatment time, whether the treatment was followed by a recovery period or not and whether cytochalasin B was used or not. Thus, these results show that CHL cells were suitable for accurately detecting clastogenic and aneugenic compounds of various types in the in vitro micronucleus test.

Published
2006
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24. Relevance of chemical structure and cytotoxicity to the induction of chromosome aberrations based on the testing results of 98 high production volume industrial chemicals.

Author

Kusakabe H, Yamakage K, Wakuri S, Sasaki K, Nakagawa Y, Watanabe M, Hayashi M, Sofuni T, Ono H, and Tanaka N

Subjects
Alcohols, Animals, Carboxylic Acids metabolism, Cell Line, Chromosomes drug effects, Cricetinae, Dose-Response Relationship, Drug, Esters metabolism, Mutagenicity Tests, Mutagens, Phenols, Phosphates metabolism, Polyploidy, Chromosome Aberrations, DNA drug effects
Abstract

Over a 6-year period (1991-1996), the chromosomal aberration testing of high production volume (HPV) industrial chemicals had been conducted using Chinese hamster lung (CHL/IU) cells according to OECD HPV testing program and the national program in Japan. A total of 98 chemicals were tested for the induction of chromosome aberration (CA), consisting of structural CA and polyploidy. Of the 98 chemicals, structural CA and/or polyploidy were induced by 39 chemicals (40%). Anilines and phenols tended to induce only structural CA. p-tert-Butylphenol had a peculiar feature in inducing not only structural CA but also polyploidy at considerably high frequency (93.2%) after continuous treatment for 48 h, posing an aneugenic potential. Not all, but six of 11 carboxylic acids or esters also showed the simultaneous induction of structural CA and polyploidy. The majority of organic phosphates, alcohols or ethers, alkyl benzenes and non-cyclic alkanes had no CA induction activity. For chemicals which were negative in the bacterial reverse mutation assay (Ames test), the proportion of the chemicals that induced CA at a severely cytotoxic dose (doses manifesting more than 50% cytotoxicity) was similar to that of the CA-negative chemicals manifesting severe cytotoxicity, suggesting that severely cytotoxic chemicals do not always induce CA.

Published
2002
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25. Induction of skin papillomas, carcinomas, and sarcomas in mice in which the connexin 43 gene is heterologously deleted.

Author

Yamakage K, Omori Y, Zaidan-Dagli ML, Cros MP, and Yamasaki H

Subjects
9,10-Dimethyl-1,2-benzanthracene pharmacology, Animals, Carcinogens pharmacology, Fibrosarcoma chemically induced, Gene Deletion, Genes, ras genetics, Mice, Mice, Inbred C57BL, Point Mutation, Skin Neoplasms chemically induced, Tetradecanoylphorbol Acetate pharmacology, Carcinoma genetics, Connexin 43 genetics, Papilloma genetics, Sarcoma genetics, Skin Neoplasms genetics
Abstract

It has been suggested that blocked gap junctional intercellular communication plays a crucial part in multistage carcinogenesis. The mouse skin tumor-promoting phorbol esters are potent inhibitors of gap junctional intercellular communication and this inhibition is considered to be a mechanism by which clonal expansion of "initiated" cells is promoted. We examined whether mice in which the gene for a gap junction protein, connexin 43, is heterozygously deleted are more susceptible to chemical carcinogenesis; connexin 43 is expressed in the basal cell layer and the dermis of the skin. When the back skin was painted with 7,12-dimethylbenz[a]anthracene and 12-O-tetradecanoylphorbol 13-acetate, the incidence and yields of both papillomas and carcinomas were similar in connexin 43+/- and connexin 43+/+ mice; for this experiment, the original mice with C57BL/6 genetic background was crossed with CD1 strain for three generations. Subcutaneous injection of 7, 12-dimethylbenz[a]anthracene resulted in induction of fibrosarcomas in connexin 43+/- and connexin 43+/+ mice to a similar extent. All papillomas and carcinomas induced with 7, 12-dimethylbenz[a]anthracene and 12-O-tetradecanoylphorbol 13-acetate contained the 7,12-dimethylbenz[a] anthracene-specific mutation in the ras gene (A to T transversion at the 61st codon). About 50% of fibrosarcomas also contained this mutation, but in the Ki-ras gene; there was no difference in the prevalence of this mutation in tumors from connexin 43+/- and connexin 43+/+ mice. None of the tumors examined, however, showed any mutation in the connexin 43 gene. These results suggest that the deletion of one allele of the connexin 43 gene does not significantly contribute to, nor alter, the molecular events involved in skin carcinogenesis. These results are compatible with previous observations that nongenetic disruption of function rather than mutations of connexins, commonly occurs in cancer cells.

Published
2000
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26. Connexins in tumour suppression and cancer therapy.

Author

Yamasaki H, Omori Y, Krutovskikh V, Zhu W, Mironov N, Yamakage K, and Mesnil M

Subjects
Animals, Connexin 26, Connexins genetics, Humans, Mutagenesis, Connexins physiology, Neoplasms genetics, Neoplasms therapy
Abstract

Malignant cells usually show altered gap junctional intercellular communication and are often associated with aberrant expression or localization of connexins. Transfection of connexin genes into tumorigenic cells restores normal cell growth, suggesting that connexins form a family of tumour suppressor genes. Some studies have also shown that specific connexins may be necessary to control growth of specific cell types. Although we have found that genes encoding connexin32 (Cx32; beta 1), Cx37 (alpha 4) and Cx43 (alpha 1) are rarely mutated in tumours, our recent studies suggest that methylation of the connexin gene promoter may be a mechanism by which connexin gene expression is down-regulated in certain tumors. We have produced various dominant negative mutants of the genes encoding Cx26 (beta 2), Cx32 and Cx43, some of which prevent the growth control exerted by the corresponding wild-type genes. A decade ago, we proposed a method to enhance killing of cancer cells by diffusion of therapeutic agents through gap junctions. Recently, we and others have shown that gap junctional intercellular communication is responsible for the bystander effect seen in herpes simplex virus thymidine kinase/ganciclovir gene therapy. Thus, connexin genes can exert dual effects in tumour control: tumour suppression and a bystander effect for cancer therapy.

Published
1999
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27. Growth control of 3T3 fibroblast cell lines established from connexin 43-deficient mice.

Author

Yamakage K, Omori Y, Piccoli C, and Yamasaki H

Subjects
3T3 Cells, Animals, Base Sequence, Blood, Cell Communication, Connexin 43 deficiency, Connexin 43 metabolism, DNA Primers, Embryo, Mammalian cytology, Female, Gap Junctions, Immunohistochemistry, Mice, Pregnancy, Cell Division genetics, Connexin 43 genetics
Abstract

Connexins are considered to be involved in cell growth control, on the basis of studies mainly with tumorigenic cells. To study the role of connexin genes in normal cell growth control, we established fibroblast cell lines from connexin 43 (Cx43)-deficient mice and characterized their growth. Embryonic fibroblasts from wild-type mice (Cx43+/+) and those with heterozygous (Cx43+/-) and homozygous (Cx43+/-) deficiencies of the Cx43 gene were cultured and passaged by a 3T3 protocol (every 3 d, 3 x 10(5) cells/60-mm dish). All cell lines showed a growth crisis during passages 6-15 and then started to grow well. All cell lines grew at similar rates under the 3T3 protocol, but Cx43-deficient (Cx43-/-) cell lines tended to grow faster when they were plated at 10(5) cells per dish. Cx43-/- cells did not express Cx43 and showed little gap-junctional intercellular communication (GJIC), confirming that Cx43 is the major connexin responsible for GJIC of these fibroblasts. While all Cx43+/+ and Cx43+/- cell lines expressed Cx43 protein, some of them showed very little GJIC. Those cell lines with high GJIC showed higher levels of the P2 form of Cx43 protein, and more Cx43 was localized in the plasma membrane than in cell lines with lower GJIC levels. We investigated effects of serum concentration on cell growth in these cell lines. Although different cell lines responded differentially to these agents, there was no clear relationship between Cx43 expression and cell growth stimulation by them. This suggests that Cx43 expression alone is not a strong regulator of mouse fibroblast growth.

Published
1998
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28. Comparative studies of MCL-5 cells and human lymphocytes for detecting indirect-acting clastogens.

Author

Yamakage K, Kusakabe H, and Tanaka N

Subjects
9,10-Dimethyl-1,2-benzanthracene pharmacokinetics, 9,10-Dimethyl-1,2-benzanthracene toxicity, Aflatoxin B1 pharmacokinetics, Aflatoxin B1 toxicity, Animals, Biotransformation, Cell Line, Cell Survival drug effects, Cyclophosphamide pharmacokinetics, Cyclophosphamide toxicity, Cytochrome P-450 Enzyme System biosynthesis, Diethylnitrosamine pharmacokinetics, Diethylnitrosamine toxicity, Dose-Response Relationship, Drug, Epoxide Hydrolases biosynthesis, Epoxide Hydrolases metabolism, Humans, Isoenzymes biosynthesis, Isoenzymes metabolism, Lymphocytes cytology, Microsomes enzymology, Microsomes, Liver metabolism, Mutagenicity Tests methods, Mutagens pharmacokinetics, Rats, Recombinant Proteins biosynthesis, Recombinant Proteins metabolism, Thymidine Kinase deficiency, Thymidine Kinase metabolism, Transfection, Chromosome Aberrations, Cytochrome P-450 Enzyme System metabolism, Lymphocytes drug effects, Mutagens toxicity
Abstract

The MCL-5 cell line was established from human lymphoblastoid TK+/- cells transfected with cDNAs of human cytochrome P450s (CYP1A2, CYP2A6, CYP2E1, and CYP3A4) and microsomal epoxide hydrolase. The TK+/- cells constitutively express a relatively high level of endogenous CYP1A1. To study metabolic activities to indirect-acting clastogens, MCL-5 cells were treated with four clastogens, i.e. aflatoxin B1 (AFB1), diethylnitrosamine (DEN), cyclophosphamide (CPA), and 7,12-dimethylbenz[a]anthracene (DMBA). Human lymphocytes from peripheral blood were used as control cells under the assay conditions with or without induced rat liver metabolic activation (S9). All chemicals tested without S9 induced chromosomal aberrations (CA) in MCL-5 cells but not in human lymphocytes. All chemicals induced CA in both cell types in the presence of S9.

Published
1998
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30. [Bullous pemphigoid].

Author

Yamakage K and Akiu N

Subjects
Adult, Aged, Aged, 80 and over, Child, Child, Preschool, Female, Humans, Male, Middle Aged, Kidney Diseases etiology, Pemphigoid, Bullous complications
Published
1997

31. Detection of neocarzinostatin-induced translocations in human sperm chromosomes using fluorescence in situ hybridization of chromosome 2.

Author

Kusakabe H, Yamakage K, and Tanaka N

Subjects
Animals, Cricetinae, Female, Humans, In Situ Hybridization, Fluorescence, Lymphocytes drug effects, Male, Mesocricetus, Chromosomes, Human, Pair 2, Mutagens toxicity, Spermatozoa drug effects, Translocation, Genetic, Zinostatin toxicity
Abstract

Mature sperm and late spermatid are known to be sensitive stages to clastogens in mammalian spermatogenesis. Certain types of chromosomal damage induced in these stages will pass to successive generations as heritable translocations. In the present study, we employed whole chromosome 2 painting with the fluorescence in situ hybridization (FISH) technique to detect the chemically induced translocations in human sperm. Mature human sperm were treated in vitro with an antitumor drug, neocarzinostatin (NCS), and fertilized in vitro with golden hamster oocytes. Sperm pronuclear chromosome slides were prepared at the first cleavage metaphase. To compare the characteristics of translocations between somatic and germ cells, human lymphocytes in peripheral blood treated with NCS in vitro were analyzed at first round metaphase after PHA-stimulation. From the analysis of translocations by whole chromosome 2 painting, frequencies of the haploid genomic translocations (FhG) were predicted for both sperm and lymphocytes. At 1.0 micrograms/ml, the actual percentages of sperm and lymphocytes with chromosome 2 translocations were almost identical (11.9% and 12.0%). At the same dose, however, the FhG of the sperm (1.15) was considerably higher than that of the lymphocytes (0.58), indicating that complex translocations having two or more rearranged sites were induced by NCS more frequently in sperm than in lymphocytes.

Published
1996
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32. Germanium poisoning: clinical symptoms and renal damage caused by long-term intake of germanium.

Author

Obara K, Saito T, Sato H, Yamakage K, Watanabe T, Kakizawa M, Tsukamoto T, Kobayashi K, Hongo M, and Yoshinaga K

Subjects
Aged, Anemia chemically induced, Child, Fatigue chemically induced, Female, Germanium administration & dosage, Germanium analysis, Hair chemistry, Humans, Intellectual Disability drug therapy, Male, Middle Aged, Nails chemistry, Gastrointestinal Diseases chemically induced, Germanium poisoning, Kidney Diseases chemically induced, Nonprescription Drugs poisoning, Peripheral Nervous System Diseases chemically induced
Abstract

We report five patients who have taken inorganic germanium preparations over a prolonged period. In all cases, the renal function deteriorated with no proteinuria or hematuria. Histological examination of the kidneys showed widespread tubular degeneration and interstitial fibrosis with minor glomerular abnormalities. Most patients had gastrointestinal symptoms such as vomiting, anorexia and weight loss; one patient had peripheral neuropathy and myopathy. A considerable amount of germanium was detected in the hair or nails of these patients. These cases clearly show that abuse of inorganic germanium compounds can induce renal damage with various extrarenal manifestations.

Published
1991
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33. Progression of experimental focal glomerulosclerosis in the spontaneously hypertensive rat.

Author

Saito T, Sato H, Obara K, Yamakage K, Abe K, Furuyama T, and Yoshinaga K

Subjects
Animals, Arteries pathology, Arterioles pathology, Blood Urea Nitrogen, Creatinine blood, Glomerulosclerosis, Focal Segmental pathology, Glomerulosclerosis, Focal Segmental physiopathology, Hypertrophy, Kidney Glomerulus blood supply, Kidney Glomerulus pathology, Male, Microscopy, Electron, Necrosis, Protamines, Proteinuria urine, Puromycin Aminonucleoside, Rats, Rats, Inbred SHR, Rats, Inbred WKY, Glomerulonephritis complications, Glomerulosclerosis, Focal Segmental complications, Hypertension complications
Abstract

To study the influence of hypertension on the progression of focal glomerulosclerosis (FGS), we produced an experimental model of FGS in spontaneously hypertensive rats (SHRs) by the combined administration of puromycinaminonucleoside (AMNS) and protamine sulfate (PS). SHRs and normotensive Wistar Kyoto rats as a control strain were given daily injections of subcutaneous AMNS (1 mg/100 gm body weight) and intravenous PS (two separated doses of 2.5 mg/100 mg body weight) for 4 days; they were killed on day 80 after three series of injections at 10-day intervals. The levels of urinary protein, serum creatinine, and urea nitrogen in SHRs given AMNS and PS were elevated throughout the experiment and were significantly higher than these levels in other control groups on day 80. Histology in SHRs given AMNS and PS showed advanced FGS associated with glomerular hypertrophy and widespread interstitial fibrosis. Most small arteries and arterioles showed "onion peel" thickening and fibrinoid necrosis of the intima, which is characteristic of malignant arteriosclerosis. We observed that the gradient of glomerulosclerosis increased from superficial to deep cortical zones; this phenomenon had often been reported in human FGS. However, these distinguished lesions were not found in control groups. Therefore, it is suggested that systemic hypertension is one of the deleterious factors enhancing histologic and functional deterioration in FGS.

Published
1990

38. The effect of protamine on proteinuria and glomerular sclerosis in aminonucleoside nephropathy.

Author

Saito T, Yamakage K, Kurosawa K, Kyogoku Y, Furuyama T, and Yoshinaga K

Subjects
Animals, Kidney Glomerulus drug effects, Male, Nephrotic Syndrome chemically induced, Rats, Rats, Inbred Strains, Sclerosis, Kidney Glomerulus pathology, Nephrotic Syndrome pathology, Protamines pharmacology, Proteinuria, Puromycin analogs & derivatives, Puromycin Aminonucleoside toxicity
Abstract

An administration of protamine sulfate combined with aminonucleoside of puromycin (AN) could produce in rats severe nephrotic syndrome and histological changes similar to focal glomerular sclerosis more distinctly than AN alone. This may be attributed to the action of protamine which seemed to enhance the effect of AN, causing polyanion loss at the glomerular basement membrane.

Published
1982
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39. The effect of protamine on serum complement activity in aminonucleoside nephropathy.

Author

Fukuda K, Seino J, Saito T, Yamakage K, Kyogoku Y, Kurosawa K, Sato H, Furuyama T, and Yoshinaga K

Subjects
Animals, Drug Interactions, Glomerulosclerosis, Focal Segmental chemically induced, Rats, Rats, Inbred Strains, Time Factors, Complement Activation drug effects, Nephrotic Syndrome chemically induced, Protamines administration & dosage, Puromycin analogs & derivatives, Puromycin Aminonucleoside administration & dosage
Abstract

Combined administration of protamine sulfate (Ps) and aminonucleoside (AN) to rats causes severe nephrotic syndrome and, histologically, focal glomerular sclerosis. These changes are more distinct than those produced by AN alone. While the exact mechanism of Ps acting on AN nephropathy is not known, marked hypocomplementemia was observed regularly after the Ps + AN injection, suggesting that complement is activated and consumed in the kidney. It is suggested that complement may play an important role in AN + Ps nephropathy.

Published
1984
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40. Focal glomerular sclerosis in aminonucleoside nephropathy.

Author

Saito T, Furuyama T, Kyogoku Y, Yamakage K, Arakawa M, and Yoshinaga K

Subjects
Animals, Disease Models, Animal, Glomerulosclerosis, Focal Segmental chemically induced, Glomerulosclerosis, Focal Segmental metabolism, Hyalin analysis, Kidney Glomerulus immunology, Kidney Glomerulus pathology, Kidney Glomerulus ultrastructure, Male, Rats, Rats, Inbred Strains, Glomerulonephritis pathology, Glomerulosclerosis, Focal Segmental pathology, Puromycin analogs & derivatives, Puromycin Aminonucleoside
Published
1981
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