Structural chromosome aberrations and sister chromatid exchanges (SCEs) in peripheral blood were studied in female workers employed in the shoe-making industry in two periods: 1987 (group I; N = 38) and 1992 (group II; N = 45). Only 11 of the workers were present in both groups and their results are presented both together and separately. Occupational exposure to benzene and toluene was confirmed through their determination in the working area, blood, and phenol in pre- and post-shift urine. The results were compared with those from the control group (N = 35). Benzene in the working atmosphere was significantly higher in 1987 compared to 1992, but was always lower than the current Croatian permissible concentration of 50 mg m-3 (in the near future this value will be changed to 15 mg m-3). A statistically significant difference was also found in biological markers of benzene exposure between the two periods of the investigation. Increased absorption in the first period occurred because of intensified production in 1987, and this decreased significantly in 1992 because of the war in Croatia. The cytogenetic study showed a significant increase in dicentric chromosomes in exposed groups I and II when compared to the control group. Statistically significant higher SCE frequencies were found in group I compared to the control group and also compared to group II. Between exposed group II and the controls no statistically significant difference in SCEs was found. Comparing the same 11 workers present in both periods the results showed no difference in chromosome aberrations between the two periods of examination. SCE frequencies were significantly higher in 1987 when greater benzene absorption occurred, confirmed by biomarkers of benzene exposure. The presented results indicate that genotoxicity may occur in workers exposed to low levels of benzene in the shoe industry.
We investigated colour vision impairment in 45 male workers occupationally exposed to toluene (mean value of toluene concentration in ambient air = 119.96 ppm) and in 53 controls. Colour vision was evaluated by Lanthony-D-15 desaturated test and expressed as Age and Alcohol Intake Adjusted Colour Confusion Score (AACDS) or types of dyschromatopsia. Exposure was evaluated by measurement of toluene concentration in ambient air and blood, and hippuric acid and orthocresol determined in urine after the workshift. A statistically significant higher AACDS value was established in the exposed subjects compared to the controls (p < 0.0001). There was no significant difference between AACDS values on Wednesday morning compared to Monday morning. In the exposed group AACDS significantly correlated with the concentration of toluene in ambient air, concentration of toluene in blood and the concentration of hippuric acid in urine after the workshift (all p < 0.0001). Dyschromatopsias were detected in both groups, although no significant difference between groups was established. In the exposed group concentration of toluene in ambient air, alcohol intake and age explained 35.1%, concentration of toluene in blood, age and alcohol intake explained 19.9%, and concentration of hippuric acid in urine and age explained 19.2% of the variation in type III dyschromatopsia. Concentration of toluene in ambient air and age explained 28.3% of the variation in total dyschromatopsia, and concentration of hippuric acid and age explained 13.8%. In the control group, age and alcohol intake explained 19.6% of the variation in type III dyschromatopsia. In exposed workers a significant difference was found in the AACDS value compared to controls. However, no significant difference was found in the prevalence of colour vision loss in the yellow-blue and/or red-green axis. Based on the results of this study the authors conclude that the effect of toluene on colour vision can be chronic and that the possible reparation period in colour vision impairment is longer than 64 hours.
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