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1. |
THE CHANGING CIGARETTE, 1950-1995 |
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Journal of Toxicology and Environmental Health,
Volume 50,
Issue 4,
1997,
Page 307-364
Dietrich Hoffmann, Ilse Hoffmann,
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摘要:
Nicotine is recognized to be the major inducer of tobacco dependence. The smoking of cigarettes as an advantageous delivery system for nicotine, accelerates and aggravates cardiovascular disease, and is causally associated with increased risks for chronic obstructive lung disease, cancer of the lung and of the upper aerodigestive system, and cancer of the pancreas, renal pelvis, and urinary bladder. It is also associated with cancer of the liver, cancer of the uterine cervix, cancer of the nasal cavity, and myeloid leukemia. In 1950, the first large-scale epidemiological studies documented that cigarette smoking induces lung cancer and described a dose-response relationship between number of cigarettes smoked and the risk for developing lung cancer. In the following decades these observations were not only confirmed by several hundreds of prospective and case-control studies but the plausibility of this causal association was also supported by bioassays and by the identification of carcinogens in cigarette smoke. Whole smoke induces lung tumors in mice and tumors in the upper respiratory tract of hamsters. The particulate matter of the smoke elicits benign and malignant tumors on the skin of mice and rabbits, sarcoma in the connective tissue of rats, and carcinoma in the lungs of rats upon intratracheal instillation. More than 50 carcinogens have been identified, including the following classes of compounds: polynuclear aromatic hydrocarbons (PAH), aromatic amines, and Nnitrosamines. Among the latter, the tobacco-specific N-nitrosamines (TSNA) have been shown to be of special significance. Since 1950, the makeup of cigarettes and the composition of cigarette smoke have gradually changed. In the United States, the sales-weighted average "tar" and nicotine yields have declined from a high of 38 mg "tar" and 2.7 mg nicotine in 1954 to 12 mg and 0.95 mg in 1992, respectively. In the United Kingdom, the decline was from about 32 mg "tar" and 2.2 mg nicotine to less than 12 mg "tar" and 1.0 mg nicotine per cigarette. During the same time, other smoke constituents changed correspondingly. These reductions of smoke yields were primarily achieved by the introduction of filter tips, with and without perforation, selection of tobacco types and varieties, utilization of highly porous cigarette paper, and incorporation into the tobacco blend of reconstituted tobacco, opened and cut ribs, and "expanded tobacco." In most countries where tobacco blends with air-cured (burley) tobacco are used, the nitrate content of the cigarette tobacco increased. In the United States nitrate levels in cigarette tobacco rose from 0.3-0.5% to 0.6-1.35%, thereby enhancing the combustion of the tobacco. More complete combustion decreases the carcinogenic PAH, yet the increased generation of nitrogen oxides enhances the formation of the carcinogenic N-nitrosamines, especially the TSNA in the smoke. However, all analytical measures of the smoke components have been established on the basis of standardized machine smoking conditions, such as those introduced by the Federal Trade Commission, that call for 1 puff to be taken once a minute over a 2-s period with a volume of 35 ml. These smoking parameters may have simulated the way in which people used to smoke the high-yield cigarettes; however, they no longer reflect the parameters applicable to contemporary smokers, and especially not those applicable to the smoking of low- and ultra-low-yield filter cigarettes. Recent smoking assays have demonstrated that most smokers of cigarettes with low nicotine yield take between 2 and 4 puffs per minute with volumes up to 55 ml to satisfy their demands for nicotine. The overview also discusses further needs for reducing the toxicity and carcinogenicity of cigarette smoke. From a public health perspective, nicotine in the smoke needs to be lowered to a level at which there is no induction of dependence on tobacco.
ISSN:0098-4108
DOI:10.1080/009841097160393
出版商:Informa UK Ltd
年代:1997
数据来源: Taylor
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2. |
TESTICULAR EFFECTS OF 1,3,5-TRINITROBENZENE (TNB). I. DOSE RESPONSE AND REVERSIBILITY STUDIES |
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Journal of Toxicology and Environmental Health,
Volume 50,
Issue 4,
1997,
Page 365-378
A. M. Sundeep Chandra, Charles W. Qualls, Jr. Gunda Reddy,
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摘要:
Testicular effects of TNB were characterized after single and multiple oral doses of TNB at 0, 35.5, and 71 mg/kg. Male Fischer 344 (F344) rats were killed after a single dose or after 4 and 10 daily doses of TNB. Testicular effects were not evident at the light microscope level in rats killed after a single dose of TNB or after 4 daily doses at 35.5 mg/kg of TNB. Rats receiving 4 daily doses of TNB at 71 mg/kg had the earliest evidence of testicular damage, with necrosis and degeneration of pachytene spermatocytes including a significant decrease in testicular weight. Rats dosed at 35.5 mg/kg for 10 d had severe testicular lesions, in addition to the decrease in testicular weight. There was degeneration of round and elongate spermatids, and formation of multinucleate syncytial cells. The epididymis was devoid of sperm, instead containing exfoliated syncytial spermatids. Rats dosed at 71 mg/kg of TNB for 10 d had testicular atrophy and cessation of spermatogenesis. These rats also had apoptic cells in the ventral prostate. To assess the extent of reversibility in these atrophied testis, rats were allowed to recover for 10 or 30 d after 10 doses of TNB (71 mg/kg). A significant regenerative attempt with proliferating spermatocytes were present at 10 d and elongate spermatids were evident at 30 d. These reversibility studies indicate testicular effects of TNB are at least partially reversible.
ISSN:0098-4108
DOI:10.1080/009841097160401
出版商:Informa UK Ltd
年代:1997
数据来源: Taylor
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3. |
TESTICULAR EFFECTS OF 1,3,5-TRINITROBENZENE (TNB). II. IMMUNOLOCALIZATION OF GERM CELLS USING PROLIFERATING CELL NUCLEAR ANTIGEN (PCNA) AS AN ENDOGENOUS MARKER |
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Journal of Toxicology and Environmental Health,
Volume 50,
Issue 4,
1997,
Page 379-388
A. M. Sundeep Chandra, Charles W. Qualls, Jr., Gregory A. Campbell Gunda Reddy,
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摘要:
The applicability of PCNA as a tool for the analysis of germ cells in rats treated with 1,3,5-trinitrobenzene (TNB), a potent testicular toxicant, was evaluated. Male Fischer 344 (F344) rats were gavaged with TNB at 71 mg/kg or with corn oil (vehicle). Rats were killed after 10 daily oral doses or were allowed to recover for 10 or 30 d after the 10 doses. Testes from control rats, treated rats, and rats allowed to recover were immunohistochemically stained for PCNA. PCNA labeling in the control rats was confined to the nuclei of spermatogonia, pachytene spermatocytes, and nuclei of elongate spermatocytes. Conventional (hematoxylin and eosin) staining of testes from rats treated with TNB at 71 mg/kg for 10 d revealed loss of germ cells and cessation of spermatogenesis. Immunohistochemical staining of sections from these treated rats revealed only PCNA-positive spermatogonia. Rats allowed a 10-d recovery had both spermatogonial and spermatocytic staining, indicating partial restoration of germ-cell population. In rats allowed to recover for 30 d, the PCNA staining pattern was identical to the control rats. These results indicate that PCNA can be used to assess the proliferative status of spermatogonia (germ cells) in rodent testes exposed to testicular toxicants.
ISSN:0098-4108
DOI:10.1080/009841097160410
出版商:Informa UK Ltd
年代:1997
数据来源: Taylor
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4. |
COMPARATIVE EFFECTS OF DISULFIRAM AND DIETHYLDITHIOCARBAMATE AGAINST TESTICULAR TOXICITY IN RATS CAUSED BY ACUTE EXPOSURE TO CADMIUM |
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Journal of Toxicology and Environmental Health,
Volume 50,
Issue 4,
1997,
Page 389-400
Hiroshige Ono Takayuki Funakoshi, Hideaki Shimada, Shoji Kojima,
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摘要:
Disulfiram (DSF) and diethyldithiocarbamate (DED) were compared for their protective effects against the testicular toxicity induced by acute exposure to cadmium (Cd) in rats. Rats were injected subcutaneously with CdCl2 [26.7 mol (3 mg) Cd/kg], and 30 min later they were injected intraperitoneally with DSF (0.05-0.5 mmol/kg) or DED (0.1-1 mmol/kg). The treatment with DSF at dose levels of 0.1-0.5 mmol/kg prevented the increases in testicular lipid peroxidation and calcium (Ca) concentrations and the decreases in testicular weight that were observed at 7 d after Cd injection. DED at dosage levels of 0.2-1 mmol/kg likewise reduced Cd-induced testicular toxicity. An increase in testicular iron (Fe) concentrations at 7 d and sterility at 59 d after Cd injection were almost completely blocked by treatment with DSF or DED at the highest doses, but lower doses of DSF or DED were ineffective. These results indicated that DSF, which is metabolized to DED, had a protective effect against Cd-induced testicular toxicity nearly equivalent to DED at approximately one-half the dose.
ISSN:0098-4108
DOI:10.1080/009841097160429
出版商:Informa UK Ltd
年代:1997
数据来源: Taylor
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5. |
DETERMINATION OF o-CRESOL BY GAS CHROMATOGRAPHY AND COMPARISON WITH HIPPURIC ACID LEVELS IN URINE SAMPLES OF INDIVIDUALS EXPOSED TO TOLUENE |
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Journal of Toxicology and Environmental Health,
Volume 50,
Issue 4,
1997,
Page 401-408
Leiliane Coelho Andre Amorim, Edna Maria Alvarez-Leite,
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摘要:
Hippuric acid is the most frequently used biomarker in the biological monitoring of occupational exposure to toluene. This product of solvent biotransformation may be also found in the urine of individuals who have not been exposed to the solvent. A smaller fraction of the absorbed toluene is oxidized to aromatic compounds including ortho-cresol, which is not found significantly in the urine of nonexposed individuals. An analytical methodology whereby gas chromatography with flame ionization detection is utilized for determination of o-cresol in urine of workers exposed to toluene is described. The levels obtained were subsequently compared to hippuric acid levels determined in the same urine samples. The analytical method has demonstrated an adequate precision (intra- and interassay coefficient of variation in the range of 2.4-5.4%) and average recovery of 98%. The samples for o-cresol determination were obtained from workers exposed to toluene in three different industrial activities. The concentration range found in exposed groups varied from <0.21 to 2.8 g/ml. The o-cresol values in the urine did not differ significantly among the exposed groups analyzed at the 5% level. The o-cresol and hippuric acid values found in the urine samples showed a significant correlation at the 1% level. These results may represent an additional contribution to studies for a definitive evaluation of the validity of ocresol as a biomarker of exposure to toluene. </abs>
ISSN:0098-4108
DOI:10.1080/009841097160438
出版商:Informa UK Ltd
年代:1997
数据来源: Taylor
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6. |
INDUCTION OF MICRONUCLEATED AND MULTINUCLEATED CELLS BY MAN-MADE FIBERS IN VITRO IN MAMMALIAN CELLS |
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Journal of Toxicology and Environmental Health,
Volume 50,
Issue 4,
1997,
Page 409-414
T. Ong, Y. Liu, B.-Z. Zhong, W. G. Jones, W.-Z. Whong,
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摘要:
Many workers as well as the general public are exposed to glass fibers, which are among the most common man-made fibers. Information related to their genotoxicity and potential carcinogenicity is still limited. In this study, we investigated the ability of glass fibers to induce micronucleated and multinucleated cells in cultured Chinese hamster lung fibroblasts, the V79 cells. The induced micronuclei were further analyzed to determine the mechanism of micronucleus formation by staining the kinetochore with anti-kinetochore and fluoresceinated goat anti-human immunoglobulin G (IgG) antibodies. Three types of glass fibers (Manville 100 microfiber, Owens Corning AAA-10 microfiber, and Owens Corning general building insulation fiber) were studied. The results show that the two microfibers induced significant numbers of multinucleated and micronucleated cells in a concentration-related manner. Immunofluorescent staining demonstrated a significant doserelated increase in the proportion of kinetochore-positive micronuclei in cells treated with the two microfibers. These results indicate that the two microfibers are capable of inhibiting cytokinesis and are principally aneuploidogens. Unlike the two microfibers, the larger fibers neither induced micronuclei nor inhibited cytokinesis in V79 cells. Thus, the genotoxic potential of glass fibers in V79 cells may be related to their size.
ISSN:0098-4108
DOI:10.1080/009841097160447
出版商:Informa UK Ltd
年代:1997
数据来源: Taylor
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