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1. Introduction

Organic solvents, a class of chemical genotoxic agents, are mainly used in petrol pumps (benzene, xylene, naphthalene, and 1,2,4-trimethylbenzene), dry cleaning (e.g., tetrachloroethylene), as paint thinners (e.g., toluene, turpentine), and so forth. The exposure of organic solvents can lead to euphoria and hallucinations while high doses may produce life-threatening effects such as convulsions and coma. The long term exposure may lead to cancer risk [1]. Paint workers utilize a variety of chemicals including dyes, solvents (thinners), and finishing chemicals. Toluene is a major solvent used in paint thinners. Given its relatively high volatility, it is predicted that 99 per cent toluene released into the environment is present in the atmosphere. Inhalation of toluene depresses the nervous system. The major effects on humans following acute exposure to high concentrations of toluene include central nervous system dysfunction and unconsciousness. Death can occur in extreme cases. Liver and kidney injury may also occur with exposure to high concentrations. Occupational exposure to moderate levels has been associated with fatigue, sleepiness, headaches, nausea, and decreased manual dexterity and visual perception.

Various kinds of biomarkers have been applied for biological monitoring of exposed population. The examples of such biomarkers include cytogenetic changes (structural and numerical changes in chromosomes, micronuclei formation, sister chromatid exchanges, etc.), somatic mutations, and changes in tumor suppressor genes. Sister chromatid exchanges (SCEs) are interchanges of DNA replication products between sister chromatids at apparently homologous loci, suggested to represent homologous recombination repair of DNA double strand breaks [2, 3]. Biomarkers of susceptibility are indicators of an inherent or acquired ability of an organism to respond to the challenge of exposure to a specific chemical substance. These biomarkers provide an indication of the extent to which an individual may be prone to progress from exposure to developing an adverse health effect. CYP2E1 and CYP1A1 genes are mainly involved in metabolism of toluene. CYP2E1 gene forms 2 alleles c1 and c2. The genotype c1/c1 was defined as type A, genotype c1/c2 as type B, and homozygote c2/c2 as type C or CYP2E1 ${}^{\ast }$ 5B [4]. The CYP2E1 genetic polymorphism varies significantly among different ethnic groups [5, 6]. The CYP1A1 gene is characterized by several polymorphisms, one of which located in exon 7 and consists of an amino acidic exchange (CYP1A1 ${}^{\ast }$ 2B or CYP1A1 m2). The variants of the CYP1A1 gene have been extensively studied, especially to evaluate their possible role in DNA damage and cancer promotion [7, 8].

2. Materials and Methods

2.1. Studied Population

The study was carried out on paint workers (30) and control group consisting of healthy individuals (30) matched with respect to age and other confounding factors except for exposure to toluene. Participants were informed of the objectives of the study. They were asked to sign an informed consent form and each participant was personally interviewed by a standard questionnaire having information related to age, personal medical history, and occupational history of exposure to paint thinners. The research protocol was approved by the Ethical Committee of Kurukshetra University, Kurukshetra, Haryana, India.

2.2. Urinary Hippuric Acid Analysis for Internal Toluene Exposure

To assess the toluene exposure in exposed population, the levels of hippuric acid in urine samples of exposed and control subjects were analyzed by colorimetric method [9].

2.3. Sample Collection

A total of 5 mL venous blood was collected from each subject in two separate vacutainer tubes containing sodium heparin and dipotassium ethylenediaminetetraacetic acid (EDTA) for lymphocyte culture setup and DNA extraction, respectively. The samples were brought to laboratory in a well-insulated icebox. All exposed individuals have minimum 2 years of working exposure. Blood samples of subjects were collected after finishing of their work shift.

2.4. Culture Setup

Short term peripheral blood lymphocytes (PBL) cultures were set up using earlier studied techniques of Moorhead et al. [10] with minor modifications. Cultures were set up in duplicate from whole blood of exposed and control group.

2.4.1. SCE in Peripheral Blood Lymphocytes (PBL)

For sister chromatid exchange (SCE) analysis, whole heparinized blood (0.4 mL) was added to 5 mL of RPMI 1640 culture medium containing 1% L-glutamine, 20% fetal bovine serum, penicillin (100 IU/mL), streptomycin (100 μg/mL), and 2% phytohaemagglutinin. 5-Bromo-2-deoxyuridine in final concentration of 10 μg/mL culture was added after 24 h of incubation. The cultures were incubated for another 48 h at 37°C and ±5% CO₂. Two drops of colchicines in a final concentration of 0.2 μg/mL was added 45 min prior to the harvesting. The cells were harvested by centrifugation and then treated with hypotonic solution (0.075 M KCl) and fixed in methanol : acetic acid (3 : 1). From a suspension of fixed cells, slides were prepared by the air drying method and stained with Hoechst 33258 and 4% Giemsa stain solution following the method of Perry and Wolff [11]. For calculating the frequency of SCE, 50 well-spread second metaphase stages were analyzed for every participant.

2.5. CYP2E1 ${}^{\ast }$ 5B Genotyping

The 5-flanking polymorphic site of the CYP2E1 gene was analyzed according to protocol of Hayashi et al. [4]. The primers F 5′-CAGTCGAGTCTACAT-TGTC-3′, R 5′ TTCATTCTGTCTTCTAACTG-3′ generated a 410 bp band. PCR products were digested with Pst1 restriction enzyme and then subjected to electrophoresis on a 2.5% agarose. The genotypes of CYP2E1 were classified as homozygous wild (c1/c1) 410 bp, heterozygote (c1/c2) 410, 290, and 120 bps, and homozygous mutant (c2/c2) 290, 120 bps. The digested PCR products were separated by 2.5% agarose gel electrophoresis and were detected by ethidium bromide staining.

2.6. CYP1A1m2 Genotyping

The primers 5′-TTC CAC CCG TTG CAG CAG GAT AGC C-3′ and 5′-CTG TCT CCC TCT GGT TAC AGG AAG-3′ [12] were used for identifying CYP1A1m2 polymorphism (204 bp). The restriction enzyme BsrDI was used to digest PCR product (204 bp) to identify mutant genotypes as later ones generate 149 and 55 bp (for the m2 site) fragments. The restricted products were analyzed by electrophoresis in 3% agarose gel containing ethidium bromide.

2.7. Statistical Analysis

Statistical analysis was performed using SPSS software package (version 16.0 for Windows; SPSS, Chicago, IL). All tests were performed in duplicate and results were expressed as means ± SD. Multivariate ANOVA test was used with post hoc analysis for the comparison of frequencies in multiple subgroups among studied population. $p<0.05$ was considered as the significant level for the statistical analyses.

3. Results

The demographic characteristics of studied population have been summarized in Table 1. We collected data from 30 occupationally exposed paint workers and 30 unexposed control subjects. The exposed workers had an average age (years) of $29.77\pm 6.52$ while mean age (years) of control subjects was $31.23\pm 6.60$ . The percentages of smokers, alcohol users, and tobacco users were 20%, 16.7%, and 6.7%. The mean value of exposure duration per day was $6.20\pm 2.93$ (hrs).

Table 1

Demographic characteristics of exposed and control population.

Student’s $t$ -test was applied for comparing mean value among control and exposed group. Chi-square test was applied for difference in consumption habits history among studied population. Level of significance was set at $p<0.05$ .

3.1. Urinary Hippuric Acid Assessment

Mean concentration of hippuric acid in urine samples of exposed subjects ( $0.43\pm 0.017$  mg/mL) was significantly higher than that of control subjects ( $0.17\pm 0.014$  mg/mL) ( $p<0.05$ ) (Figure 1).

3.2. SCE Frequency in Control and Exposed Group

In paint workers mean frequency of SCE was found to be significantly higher ( $4.81\pm 0.92$ ) than control population ( $1.73\pm 0.54$ ) (Figure 2).

Workers having >6 years of exposure duration had significant high SCE frequency ( $5.46\pm 0.72$ ) compared to individuals having <6 years of exposure ( $4.32\pm 0.73$ ) (Figure 3).

3.3. SCE Frequency by Age and Consumption Habits

Individuals being >40 years were found to have significant higher SCE frequency in exposed and control population ( $5.83\pm 0.62$ ; $1.95\pm 0.29$ ), respectively (Table 2). There was nonsignificant but high SCE frequency showed in nonsmokers ( $4.85\pm 0.92$ ); alcoholics ( $5.05\pm 1.27$ ); and nontobacco users ( $5.49\pm 0.38$ ) in exposed population.

Table 2

SCE frequency by age and consumption habits.

${}^{\ast }$ Significant at $p<0.05$ ; multivariate ANOVA test was used with post hoc analysis for the comparison in SCE frequency in multiple subgroups among studied population.

${}^{\ast \mathrm{\yen }}$ Significant at $p<0.05$ + highest mean rank; ^¥highest mean rank (Kruskal-Wallis $H$ test).

3.4. Influence of CYP Genotypes on SCE Frequency

CYP1A1m2 homozygous mutants showed significant difference in SCE frequency in exposed ( $5.61\pm 0.66$ ) and control group ( $2.36\pm 0.00$ ). CYP2E1 homozygous mutants (mt/mt) in exposed subjects ( $6.11\pm 0.08$ ) and heterozygous mutants (wt/mt) in control subjects ( $1.88\pm 0.45$ ) showed high SCE frequency (Table 3).

Table 3

Influence of CYP genotypes on SCE frequency.

${}^{\ast }$ Significant at $p<0.05$ ; multivariate ANOVA test was used for the comparison in SCE frequency in multiple subgroups among studied population.

Results of linear regression analysis, adjusted for model such as age, gender, exposure, and consumption habits, have been shown in Table 4.

Table 4

Influence of CYP genotypes on SCE as analyzed by linear regression.

${}^{\mathrm{a}}$ Unstandardised coefficient.

${}^{\mathrm{b}}$ Model $p$ value. Regression analysis was used for the differences in SCE frequency adjusted for age, exposure duration, and consumption habits.

4. Discussion

In present study we found that exposed population has significantly high SCE frequency compared to that of control. Popp et al. [13] investigated the frequency of DNA strand breakage and crosslinking and sister chromatid exchange frequency in the lymphocytes of female workers exposed to benzene and toluene. In the female workers significantly raised ( $p<0.05$ ) SCE values were found. In a study among 25 male public building painters aged between 18 and 62 years in Mexico, increased SCE levels in lymphocytes were found when compared to the same number of sex- and age-matched unexposed controls [14]. Further, SCEs were evaluated in 25 car painters working in different automobile paint shops in Italy and 37 unexposed control subjects (healthy blood donors). The exposed workers had higher frequencies of SCEs than controls ( $p<0.05$ ) [15]. Contradicting our results, Haglund et al. [16] studied chromosome aberrations and sister chromatid exchanges in Swedish paint industry workers exposed to a mixture of organic solvents, mainly containing xylene or toluene. No difference in the frequency of sister chromatid exchanges (SCEs) was noted in the peripheral lymphocytes of the exposed group of 17 workers and their matched reference group. Our results showed that there was significant increase in frequencies of SCE among the mutant genotypes of CYP2E1 and CYP1A1m2 as compared to wild genotypes. Similar to our results, Kezic et al. [17] studied polymorphisms in the genes encoding CYP1A1, CYP2E1, EPHX1, GSTM1, GSTT1, and GSTP1 enzymes in a group of male CSE (chronic solvent encephalopathy) patients ( $N=97$ ) and controls ( $N=214$ ). Comparing patients and controls, higher frequencies of the variant ${}^{\ast }$ 5B allele of the CYP2E1 gene and of the variant GSTP1 ${}^{\ast }$ C allele were found.

5. Conclusion

In our study, we have found that CYP2E1 and CYP1A1m2 gene modulate the genotoxic effects in paint workers. The determination of CYP2E1 and CYP1A1m2 genotypes status could also be helpful in providing baseline data as an individual marker of susceptibility in exposed population. It is recommended that occupational paint workers are required to train regularly and always be given appropriate personal protective equipment.

Acknowledgments

The authors are thankful to Kurukshetra University for grant of University Research Fellowship to the first author and to all blood donors. They are also grateful to Mr. Rajesh, Statistical Officer at Department of Forensic Sciences, Postgraduate Institute of Medical Education and Research, Chandigarh, Haryana (India), for statistical analysis.