Abstract
Background
Previous studies have suggested that polycyclic aromatic hydrocarbons (PAHs) may be associated with breast cancer. However, the carcinogenicity of PAHs on the human breast remains unclear. Certain carcinogens may be associated with specific mutation patterns in the p53 tumor suppressor gene, thereby contributing information about disease etiology.
Objectives
We hypothesized that associations of PAH-related exposures with breast cancer would differ according to tumor p53 mutation status, effect, type, and number.
Methods
We examined this possibility in a population-based case–control study using polytomous logistic regression. As previously reported, 151 p53 mutations among 859 tumors were identified using Surveyor nuclease and confirmed by sequencing.
Results
We found that participants with p53 mutations were less likely to be exposed to PAHs (assessed by smoking status in 859 cases and 1,556 controls, grilled/smoked meat intake in 822 cases and 1,475 controls, and PAH–DNA adducts in peripheral mononuclear cells in 487 cases and 941 controls) than participants without p53 mutations. For example, active and passive smoking was associated with p53 mutation–negative [odds ratio (OR) = 1.55; 95% confidence interval (CI), 1.11–2.15] but not p53 mutation–positive (OR = 0.77; 95% CI, 0.43–1.38) cancer (ratio of the ORs = 0.50, p < 0.05). However, frameshift mutations, mutation number, G:C→A:T transitions at CpG sites, and insertions/deletions were consistently elevated among exposed subjects.
Conclusions
These findings suggest that PAHs may be associated with specific breast tumor p53 mutation subgroups rather than with overall p53 mutations and may also be related to breast cancer through mechanisms other than p53 mutation.
Keywords: breast cancer, p53 mutation, p53 overexpression, PAH, polycylic aromatic hydrocarbons
Breast cancer is the second leading cancer-related cause of death among women in the United States (American Cancer Society 2008). Previous epidemiologic and experimental investigations suggest that polycyclic aromatic hydrocarbons (PAHs) may be associated with breast cancer (Bonner et al. 2005; el-Bayoumy et al. 1995; Gammon et al. 2002b, 2004b; Rundle et al. 2000). However, despite strongly positive associations in animal models and some evidence of a positive association in humans, the carcinogenicity of these chemical compounds on the human breast remains unclear.
PAHs are ubiquitous environmental pollutants formed by incomplete combustion of organic material (Samanta et al. 2002). These chemicals have estrogenic properties (Santodonato 1997), are known carcinogens in humans (Samanta et al. 2002), and cause mammary tumors in laboratory animals (el-Bayoumy et al. 1995; Hecht 2002). Exposure to PAHs in the general population occurs primarily through charred, smoked, and broiled foods; leafy vegetables (Phillips 1999); wood- and coal-burning stoves (Lewis et al. 1999); air pollution (Lioy and Greenberg 1990); and tobacco smoke (Besaratinia et al. 2002). PAH–DNA adducts (Gammon et al. 2004b), lifetime intake of grilled/smoked meat (Steck et al. 2007), and long-term passive smoking—but not current or former active smoking (Gammon et al. 2004a)—have been associated with breast cancer in our study population.
Cigarette smoke is associated with PAH–DNA adducts in human lymphocytes (Shantakumar et al. 2005), and the PAH benzo[a]pyrene (B[a]P) from cigarette smoke induces neoplastic transformation of human breast epithelial cells (Russo et al. 2002). However, smoking has been inconsistently linked to breast cancer in epidemiologic research, with more consistently positive findings reported for long-term passive smoking and among genetically susceptible subgroups (Ambrosone et al. 2008; Terry and Goodman 2006; Terry and Rohan 2002).
PAHs are formed on the surface of “well-done” meat (Kazerouni et al. 2001), but epidemiologic studies examining meat intake or doneness have yielded inconclusive results (Holmes et al. 2003; Zheng et al. 1998). These studies have primarily focused on recent dietary habits, whereas lifetime intake may be more relevant for carcinogenesis. Steck et al. (2007) observed a positive association between lifetime intake of grilled and smoked meat and breast cancer among postmenopausal women [middle vs. lowest tertile of intake, odds ratio (OR) = 1.47; 95% confidence interval (CI), 1.11–1.95; highest vs. lowest tertile of intake, OR = 1.47; 95% CI, 1.12–1.92)].
PAHs are metabolized through activation and detoxification pathways. When PAH exposure is high or detoxification is insufficient, PAH–DNA adducts form, including in breast tissue (Gammon and Santella 2008; Santella 1999). Adducts persist when repair mechanisms are inadequate (Braithwaite et al. 1999). Therefore, PAH–DNA adducts reflect both exposure to PAHs and host response—which differs because of variation in metabolism and/or DNA repair capacity between individuals—and are consistently associated with breast cancer in epidemiologic research (Gammon and Santella 2008).
The p53 protein is a transcription factor that regulates cell proliferation, differentiation, apoptosis, and DNA repair and therefore plays an important role in normal cell function and neoplastic transformation (Levine 1997). Certain carcinogens may be associated with specific mutation patterns in the p53 tumor suppressor gene, and these characteristic patterns of DNA damage may contribute information about disease etiology by lending biologic support to exposure–disease associations and by helping to evaluate potential mechanisms of carcinogenesis (Greenblatt et al. 1994). Smoking has been associated with breast tumor p53 mutational spectra (Conway et al. 2002). We hypothesized that associations between PAH-related exposures and breast cancer would differ according to tumor p53 mutation status, effect, type, and number and we investigated this possibility using data from a population-based study.
Materials and Methods
Study population
Study subjects were participants from the Long Island Breast Cancer Study Project (LIBCSP), details of which have been published previously (Gammon et al. 2002a). Briefly, the LIBCSP is a population-based case–control study conducted among English-speaking women 20–98 years of age residing in Nassau and Suffolk counties in Long Island, New York. Cases were newly diagnosed with a first primary in situ or invasive breast cancer between 1996 and 1997, and were identified by rapid case ascertainment through contact with local pathology departments. Controls with no history of breast cancer were randomly selected from the same two counties using random digit dialing for women < 65 years of age and by Health Care Finance Administration rosters for women > 65 years of age. Controls were frequency matched to the expected age distribution of cases by 5-year age group. A total of 1,508 cases and 1,556 controls (82.1% and 62.7%, respectively, of all eligible subjects) completed the interview.
Questionnaire assessment of PAH exposures
Trained interviewers completed in-home questionnaires with cases and controls. Questionnaire topics included reproductive history, annual household income, alcohol intake, race, education, active and passive cigarette smoking, lifetime dietary consumption of grilled and smoked foods, and other lifestyle factors. Ninety-eight percent of cases and 98% of controls completed a self-administered modified Block food frequency questionnaire (Block et al. 1986). These assessments were used to estimate lifetime intake of grilled and smoked meat, active and passive smoking, and daily intakes of B[a]P from meat and total energy using previously described methods (Gammon et al. 2004a; Steck et al. 2007).
PAH–DNA adducts
Seventy-three percent of cases and 73% of controls donated a blood sample at the interview (Gammon et al. 2002a). DNA extracted from blood samples was used to assess PAH–DNA adduct levels in whole blood by competitive enzyme-linked immunosorbent assay (Gammon et al. 2002b). The antibody used in this analysis recognizes PAH diol epoxide adducts that form at the N2 position of guanine.
p53 mutation analysis
Archived paraffin-embedded tumor tissue was obtained from participating hospitals for 67% of case participants. DNA was successfully extracted from tumor tissue for 859 women, and mutations were detected in exons 5–8 of p53 through a multistep process (Rossner et al. 2008). Briefly, the samples were amplified using polymerase chain reaction (PCR), and the Surveyor Mutation Detection Kit (Transgenomic, Omaha, NE, USA) was used as a screening method for detection of p53 mutations. Samples screening positive for potential mutations were selected for confirmation and identification of mutations by PCR amplification and sequencing using an ABI 3100 capillary sequencer (Applied Biosystems Inc., Foster City, CA, USA). Surveyor nuclease shows some single-base mismatch cutting preference, although this disadvantage may be ameliorated by formation of alternate heteroduplex mismatches (Qiu et al. 2004). As previously reported by Rossner et al. (2008), we identified a total of 151 p53 mutations among 859 tumors, with 15 tumors harboring multiple mutations. In total, 15% of tumors contained one or more p53 mutations, 83% of which were point mutations and 17% of which were insertions/deletions.
p53 protein overexpression by immunohistochemistry
A total of 859 cases with available tumor tissue were evaluated for p53 protein expression by immunohistochemical staining using p53 mouse monoclonal antibody clone DO-1 (Immunotech, Inc., Westbrook, ME, USA) at 1:5 dilution (Rossner et al. 2008). We evaluated nuclear staining by a semiquantitative scoring system for intensity and percentage of positive nuclei. Tumors were considered positive if the staining had an intensity score of moderate or strong, if both study pathologists considered them positive, and if at least 10% of cells showed evidence of p53 protein expression. Previously published results from the LIBCSP show p53 overexpression in 36% of tumor samples (Rossner et al. 2008).
Statistical methods
We used polytomous logistic regression (Hosmer and Lemeshow 1989) to estimate ORs and 95% CIs for associations between breast cancer categorized by p53 tumor mutation subtype and smoking, intake of PAH food sources, and PAH–DNA adducts. We evaluated whether results for p53 mutation–negative and p53 mutation–positive tumors differed statistically by calculating ratios of the ORs for the two outcomes (Schlesselman 1982). Polytomous logistic regression (Hosmer and Lemeshow 1989) was also used to estimate the ORs and 95% CIs for associations between breast cancer categorized by tumor p53 protein expression status and these same PAH-related factors. Because cases and controls were frequency matched by 5-year age group, we adjusted all statistical models for age group at reference. We performed additional analyses to examine associations of active smoking, grilled and smoked meat intake, and a combined measure of these factors with p53 mutation status, type, and effect using referent groups consisting of never smokers with low lifetime grilled and smoked meat intake.
We defined current smokers as women who smoked within 12 months of the reference date. Former smokers stopped smoking > 12 months before this date, and passive smokers were women who reported ever living with an active smoker (Gammon et al. 2004a). We categorized lifetime intake of grilled and smoked meat relative to the median intake of 4,160 lifetime servings among controls (Steck et al. 2007). Daily intake of B[a]P from meat was categorized relative to the median intake of 0.42 ng/day (Steck et al. 2007). PAH–DNA adducts were categorized as detectable or nondetectable; for analytical purposes, we categorized samples with < 15% inhibition as nondetectable (Gammon et al. 2002b).
We identified potential confounders by a thorough review of the relevant literature and analysis of causal diagrams (Shrier and Platt 2008). For PAH–DNA adducts, potential confounders were age at menarche, income, smoking status, and grilled and smoked meat intake. For dietary PAH intake, potential confounders were income, race, and energy intake. For smoking, potential confounders were income, alcohol intake, and education. We evaluated confounding by these covariates using backward selection with a 10% change in estimate criterion. In addition to adjustment for 5-year age group, we adjusted final models for daily alcohol intake when looking at smoking and age at menarche when looking at PAH–DNA adducts.
When examining associations with p53 mutation status, participants were cases and controls with complete information regarding the exposure of interest and mutation status. As previously reported, the distribution of known and suspected breast cancer risk factors did not vary substantially between cases with and without available tumor tissue for p53 mutation detection and p53 overexpression analysis (Rossner et al. 2008). Final sample sizes included 487 cases and 941 controls when examining PAH–DNA adducts, 859 cases and 1,556 controls for smoking status, and 822 cases and 1,475 controls for meat intake. Inclusion criteria and sample sizes were similar when examining associations with p53 protein expression status.
Results
The distribution of p53 mutations by smoking history, grilled and smoked meat intake, and PAH–DNA adducts is presented in Table 1, and associations between PAH-related exposures and p53 mutation status are presented in Table 2. p53 mutation–negative breast cancer was positively associated with detectable adducts (OR = 1.33; 95% CI, 1.02–1.73), active and passive smoking (OR = 1.55; 95% CI, 1.11–2.15), passive smoking from a spouse (OR = 1.25; 95% CI, 1.01–1.54), and high lifetime intake of grilled and smoked meat (OR = 1.51; 95% CI, 1.25–1.82). Effect estimates for all PAH-related exposures were elevated above the null for p53 mutation–negative cancer.
Table 1.
Distribution of p53 mutations by PAH-related exposures among LIBCSP case participants [n (%)].
Cigarette smoking history (n = 859) |
Grilled and smoked meat intakea (n = 822) |
Detectable PAH–DNA adducts (n = 487) |
||||
---|---|---|---|---|---|---|
Mutation | Ever | Never | High | Low | Yes | No |
Point mutations | ||||||
Transitions | ||||||
G:C→A:T at CpG | 23 (29.1) | 12 (16.7) | 22 (28.2) | 12 (17.1) | 16 (27.1) | 5 (23.8) |
G:C→A:T at non-CpG | 19 (24.1) | 27 (37.5) | 19 (24.4) | 27 (38.6) | 17 (28.8) | 7 (33.3) |
A:T→G:C | 7 (8.9) | 8 (11.1) | 6 (7.7) | 9 (12.9) | 7 (11.9) | 3 (14.3) |
Transversions | ||||||
G:C→T:A | 5 (6.3) | 12 (16.7) | 9 (11.5) | 6 (8.6) | 5 (8.5) | 1 (4.8) |
G:C→C:G | 5 (6.3) | 1 (1.4) | 4 (5.1) | 2 (2.9) | 1 (1.7) | 1 (4.8) |
A:T→T:A | 3 (3.8) | 2 (2.8) | 2 (2.6) | 3 (4.3) | 1 (1.7) | 2 (9.5) |
A:T→C:G | 0 (0) | 1 (1.4) | 0 (0) | 1 (1.4) | 0 (0) | 0 (0) |
Insertions or deletions | 17 (21.5) | 9 (12.5) | 16 (20.5) | 10 (14.3) | 12 (20.3) | 2 (9.5) |
Base change | ||||||
C→T at CpG | 13 (21.0) | 6 (9.5) | 12 (19.4) | 6 (10.0) | 11 (23.4) | 2 (10.5) |
G→A at CpG | 10 (16.1) | 6 (9.5) | 10 (16.1) | 6 (10.0) | 5 (10.6) | 3 (15.8) |
C→T at non-CpG | 11 (17.7) | 20 (31.8) | 15 (24.2) | 16 (26.7) | 12 (25.5) | 4 (21.1) |
G→A at non-CpG | 8 (12.9) | 7 (11.1) | 4 (6.5) | 11 (18.3) | 5 (10.6) | 3 (15.8) |
T→C | 3 (4.8) | 5 (7.9) | 3 (4.8) | 5 (8.3) | 3 (6.4) | 1 (5.3) |
A→G | 4 (6.5) | 3 (4.8) | 3 (4.8) | 4 (6.7) | 4 (8.5) | 2 (10.5) |
G→T | 1 (1.6) | 11 (17.5) | 6 (9.7) | 5 (8.3) | 2 (4.3) | 1 (5.3) |
C→A | 4 (6.5) | 1 (1.6) | 3 (4.8) | 1 (1.7) | 3 (6.4) | 0 (0) |
G→C | 3 (4.8) | 1 (1.6) | 3 (4.8) | 1 (1.7) | 0 (0) | 1 (5.3) |
C→G | 2 (3.2) | 0 (0) | 1 (1.6) | 1 (1.7) | 1 (2.1) | 0 (0) |
T→A | 1 (1.6) | 2 (3.2) | 0 (0) | 3 (5.0) | 1 (2.1) | 1 (5.3) |
A→T | 2 (3.2) | 0 (0) | 2 (3.2) | 0 (0) | 0 (0) | 1 (5.3) |
T→G | 0 (0) | 1 (1.6) | 0 (0) | 1 (1.7) | 0 (0) | 0 (0) |
Mutation effect | ||||||
Missense | 38 (48.1) | 42 (58.3) | 41 (52.6) | 36 (51.4) | 23 (39.0) | 18 (85.7) |
Nonsense | 8 (10.1) | 8 (11.1) | 7 (9.0) | 9 (12.9) | 6 (10.2) | 1 (4.8) |
Silent | 16 (20.3) | 13 (18.1) | 14 (18.0) | 15 (21.4) | 18 (30.5) | 0 (0) |
Frameshift | 17 (21.5) | 9 (12.5) | 16 (20.5) | 10 (14.3) | 12 (20.3) | 2 (9.5) |
No. of mutations | 79 | 72 | 78 | 70 | 59 | 21 |
Tumors with mutations | 66 (13.8) | 62 (16.4) | 63 (13.2) | 62 (17.9) | 47 (13.0) | 18 (14.4) |
Tumors with no mutations | 414 (86.3) | 317 (83.6) | 413 (86.8) | 284 (82.1) | 315 (87.0) | 107 (85.6) |
Total no. of tumors | 480 | 379 | 476 | 346 | 362 | 125 |
Lifetime intake of grilled and smoked meat is dichotomized based on median lifetime servings among controls (median = 4,160 servings).
Table 2.
Associations between PAH-related exposures and the risk of breast cancer subtype as defined by p53 mutation status in the LIBCSP.a
OR (95% CI) |
|||
---|---|---|---|
Mutation status | Cases/controls (n) | Age-adjusted | Multivariate-adjusted |
PAH–DNA adducts (detectable vs. nondetectable) | |||
p53+ breast cancer | 65/941 | 1.16 (0.66–2.04) | 1.28 (0.71–2.31) |
p53− breast cancer | 422/941 | 1.34 (1.03–1.75) | 1.33 (1.02–1.73) |
Ratio of the ORs (p53+ vs. p53−) | 0.86 (0.48–1.55) | 0.96 (0.52–1.78) | |
Ever active smoking versus never active smoking | |||
p53+ breast cancer | 128/1,556 | 0.90 (0.62–1.30) | 0.96 (0.66–1.39) |
p53− breast cancer | 731/1,556 | 1.11 (0.92–1.32) | 1.09 (0.91–1.31) |
Ratio of the ORs (p53+ vs. p53−) | 0.82 (0.56–1.19) | 0.88 (0.60–1.29) | |
Current active smoking versus never active smoking | |||
p53+ breast cancer | 80/989 | 0.80 (0.46–1.40) | 0.87 (0.50–1.54) |
p53− breast cancer | 468/989 | 1.22 (0.96–1.56) | 1.21 (0.94–1.55) |
Ratio of the ORs (p53+ vs. p53−) | 0.66 (0.37–1.17) | 0.72 (0.40–1.29) | |
Past active smoking versus never active smoking | |||
p53+ breast cancer | 110/1,262 | 0.97 (0.65–1.44) | 1.03 (0.69–1.55) |
p53− breast cancer | 580/1,262 | 1.06 (0.86–1.29) | 1.05 (0.85–1.29) |
Ratio of the ORs (p53+ vs. p53−) | 0.91 (0.60–1.39) | 0.99 (0.65–1.51) | |
Both active and passive smoking versus never passive or active smoking | |||
p53+ breast cancer | 68/875 | 0.71 (0.40–1.25) | 0.77 (0.43–1.38) |
p53− breast cancer | 417/875 | 1.58 (1.14–2.18) | 1.55 (1.11–2.15) |
Ratio of the ORs (p53+ vs. p53−) | 0.45 (0.24–0.82) | 0.50 (0.27–0.93) | |
Active smoking only versus never passive or active smoking | |||
p53+ breast cancer | 35/328 | 1.14 (0.55–2.38) | 1.23 (0.58–2.62) |
p53− breast cancer | 129/328 | 1.33 (0.86–2.04) | 1.44 (0.93–2.24) |
Ratio of the ORs (p53+ vs. p53−) | 0.86 (0.39–1.87) | 0.86 (0.39–1.90) | |
Ever passive smoking only versus never passive or active smoking | |||
p53+ breast cancer | 61/681 | 0.90 (0.50–1.61) | 0.94 (0.52–1.68) |
p53− breast cancer | 306/681 | 1.38 (0.99–1.91) | 1.38 (0.99–1.91) |
Ratio of the ORs (p53+ vs. p53−) | 0.65 (0.35–1.21) | 0.68 (0.37–1.27) | |
Ever passively exposed to spouse versus never passively exposed to spouse | |||
p53+ breast cancer | 93/1,228 | 1.64 (1.03–2.60) | 1.64 (1.03–2.61) |
p53− breast cancer | 602/1,228 | 1.25 (1.01–1.54) | 1.25 (1.01–1.54) |
Ratio of the ORs (p53+ vs. p53−) | 1.31 (0.81–2.12) | 1.32 (0.82–2.13) | |
Lifetime intake of smoked/grilled meat (high vs. low)b | |||
p53+ breast cancer | 125/1,475 | 1.08 (0.74–1.57) | 1.08 (0.74–1.57) |
p53− breast cancer | 697/1,475 | 1.51 (1.25–1.82) | 1.51 (1.25–1.82) |
Ratio of the ORs (p53+ vs. p53−) | 0.72 (0.48–1.06) | 0.72 (0.48–1.06) | |
Total B[a]Ps from meat (high intake vs. low intake)c | |||
p53+ breast cancer | 124/1,473 | 1.28 (0.88–1.87) | 1.28 (0.88–1.87) |
p53− breast cancer | 700/1,473 | 1.04 (0.86–1.25) | 1.04 (0.86–1.25) |
Ratio of the ORs (p53+ vs. p53−) | 1.24 (0.84–1.83) | 1.24 (0.84–1.83) |
In addition to adjustment for age group, final models were adjusted for daily alcohol intake when examining smoking exposure and age at menarche when examining PAH–DNA adducts. Ratios of the ORs [OR for the association between exposure and p53-positive (p53+) breast cancer divided by OR for the association between exposure and p53-negative (p53−) breast cancer] were calculated as indicators of heterogeneity of effects across groups.
Lifetime intake of grilled and smoked meat is dichotomized based on median lifetime servings among controls (median, 4,160 servings).
Daily intake of B[a]Ps from meat is dichotomized based on median daily intake among controls (median, 0.42 ng/day).
In contrast, many PAH-related exposures were inversely associated with p53 mutation–positive cancer (which primarily comprised missense mutations, but also included silent, nonsense, and frameshift mutations), and nearly all effect estimates for p53 mutation–positive cancer for a given exposure were lower than the corresponding effect estimate for p53 mutation–negative cancer (Table 2). Calculating ratios of the ORs (OR for the association between exposure and p53 mutation–positive breast cancer divided by OR for the association between exposure and p53 mutation–negative breast cancer) as an indicator of heterogeneity of ORs across groups yielded statistically significant differences when examining active and passive smoking exposure [p53 mutation–positive cancer: OR = 1.55 (95% CI, 1.11–2.15); p53 mutation– negative cancer: OR = 0.77 (95% CI, 0.43–1.38); ratio of the ORs, 0.50 (95% CI, 0.27–0.93)]. When we defined p53 status by protein expression status, we found no substantial heterogeneity in the ORs for the associations between PAH-related exposures and p53-positive cancer and the corresponding PAH exposures and p53-negative breast cancer [all p-values > 0.05 for the ratios of the ORs; see Supplemental Material, Table 3 (doi:10.1289/ehp.0901233)].
Associations between PAH-related exposures and selected p53 mutation types are presented in Table 3. We were unable to statistically evaluate relations for all mutation types because of small numbers of certain mutations. We found consistently elevated associations between PAH-related exposures and G:C→A:T transitions at CpG sites as well as insertions/deletions. PAH-related exposures showed different directions of association with G:C→A:T transitions at non-CpG sites (Table 3), A:T→G:C transitions, and G:C→T:A transversions (data not shown). PAH exposures were also inconsistently related to p53 missense, nonsense, and silent mutations (Table 4). Frameshift mutations were consistently associated with PAH-related exposures, and these associations were strongest for PAH–DNA adducts. Few effect estimates for mutation type or effect reached statistical significance.
Table 3.
Associations between PAH-related exposures and the risk of breast cancer subtype as defined by p53 mutation type in the LIBCSP.a
OR (95% CI) |
|||
---|---|---|---|
Mutation type | Cases/controls (n) | Age adjusted | Multivariate adjusted |
G:C→A:T at CpG transitions | |||
PAH–DNA adducts | |||
Nondetectable | 5/293 | 1.0 | 1.0 |
Detectable | 16/648 | 1.51 (0.55–4.19) | 1.53 (0.55–4.23) |
Smoking status | |||
Never | 12/698 | 1.0 | 1.0 |
Former | 16/564 | 1.60 (0.74–3.44) | 1.65 (0.76–3.58) |
Current | 6/291 | 1.33 (0.49–3.67) | 1.53 (0.55–4.27) |
Grilled and smoked meatb | |||
Low lifetime intake | 12/739 | 1.0 | 1.0 |
High lifetime intake | 21/736 | 1.69 (0.82–3.52) | 1.69 (0.82–3.52) |
G:C→A:T at non-CpG transitions | |||
PAH–DNA adducts | |||
Nondetectable | 6/293 | 1.0 | 1.0 |
Detectable | 15/648 | 1.10 (0.42–2.89) | 1.09 (0.41–2.85) |
Smoking status | |||
Never | 24/698 | 1.0 | 1.0 |
Former | 14/564 | 0.73 (0.37–1.44) | 0.80 (0.40–1.58) |
Current | 4/291 | 0.44 (0.15–1.29) | 0.51 (0.17–1.52) |
Grilled and smoked meat | |||
Low intake | 25/739 | 1.0 | 1.0 |
High intake | 17/736 | 0.72 (0.38–1.37) | 0.72 (0.38–1.37) |
Insertions/deletions | |||
PAH–DNA adducts | |||
Nondetectable | 2/293 | 1.0 | 1.0 |
Detectable | 12/648 | 2.64 (0.58–11.91) | 4.77 (0.63–36.25) |
Smoking status | |||
Never | 9/698 | 1.0 | 1.0 |
Former | 10/564 | 1.45 (0.58–3.65) | 1.44 (0.56–3.69) |
Current | 7/291 | 2.11 (0.75–5.95) | 2.41 (0.85–6.85) |
Grilled and smoked meat | |||
Low intake | 10/739 | 1.0 | 1.0 |
High intake | 16/736 | 1.68 (0.74–3.78) | 1.68 (0.74–3.78) |
In addition to adjustment for age group, final models were adjusted for daily alcohol intake when examining smoking exposure and age at menarche when examining PAH–DNA adducts.
Lifetime intake of grilled and smoked meat is dichotomized based on median lifetime servings among controls (median, 4,160 servings).
Table 4.
Associations between PAH-related exposures and the risk of breast cancer subtype as defined by p53 mutation effect in the LIBCSP.a
OR (95% CI) |
|||
---|---|---|---|
Mutation effect | Cases/controls (n) | Age adjusted | Multivariate adjusted |
Missense mutations | |||
PAH–DNA adducts | |||
Nondetectable | 15/293 | 1.0 | 1.0 |
Detectable | 20/648 | 0.62 (0.31–1.24) | 0.67 (0.33–1.36) |
Active smoking status | |||
Never | 37/698 | 1.0 | 1.0 |
Former | 26/564 | 0.87 (0.52–1.47) | 0.92 (0.54–1.56) |
Current | 7/291 | 0.51 (0.22–1.18) | 0.53 (0.23–1.24) |
Grilled/smoked meatb | |||
Low lifetime intake | 33/739 | 1.0 | 1.0 |
High lifetime intake | 34/736 | 1.09 (0.66–1.80) | 1.09 (0.66–1.80) |
Nonsense mutations | |||
PAH–DNA adducts | |||
Nondetectable | 1/293 | 1.0 | 1.0 |
Detectable | 6/648 | 2.57 (0.31–21.47) | 2.60 (0.31–21.94) |
Active smoking status | |||
Never | 8/698 | 1.0 | 1.0 |
Former | 7/564 | 1.05 (0.37–2.94) | 1.21 (0.42–3.48) |
Current | 1/291 | 0.39 (0.05–3.28) | 0.42 (0.05–3.56) |
Grilled/smoked meat | |||
Low intake | 9/739 | 1.0 | 1.0 |
High intake | 7/736 | 0.84 (0.30–2.33) | 0.84 (0.30–2.33) |
Silent mutations | |||
PAH–DNA adducts | |||
Nondetectable | 0/293 | 1.0 | 1.0 |
Detectable | 15/648 | — | — |
Active smoking status | |||
Never | 11/698 | 1.0 | 1.0 |
Former | 9/564 | 1.01 (0.41–2.48) | 1.17 (0.47–2.90) |
Current | 4/291 | 1.15 (0.35–3.78) | 1.37 (0.42–4.54) |
Grilled/smoked meat | |||
Low intake | 15/739 | 1.0 | 1.0 |
High intake | 9/736 | 0.65 (0.28–1.53) | 0.65 (0.28–1.53) |
Frameshift mutations | |||
PAH–DNA adducts | |||
Nondetectable | 2/293 | 1.0 | 1.0 |
Detectable | 12/648 | 2.62 (0.58–11.80) | 4.85 (0.62–37.75) |
Active smoking status | |||
Never | 9/698 | 1.0 | 1.0 |
Former | 10/564 | 1.44 (0.57–3.63) | 1.43 (0.56–3.66) |
Current | 7/291 | 2.11 (0.75–5.96) | 2.40 (0.84–6.85) |
Grilled/smoked meat | |||
Low intake | 10/739 | 1.0 | 1.0 |
High intake | 16/736 | 1.68 (0.75–3.79) | 1.68 (0.75–3.79) |
In addition to adjustment for age group, final models were adjusted for daily alcohol intake when examining smoking exposure and age at menarche when examining PAH–DNA adducts.
Lifetime intake of grilled and smoked meat is dichotomized based on median lifetime servings among controls (median, 4,160 servings).
Table 5 shows relations between PAH-related exposures and the number of tumor p53 mutations. We found that many PAH-related exposures were associated with higher mutation number. For example, for detectable PAH–DNA adducts, ORs were 1.19 (95% CI, 0.63–2.25) for one mutation, 1.87 (95% CI, 0.38–9.20) for two mutations, and 2.15 (95% CI, 0.59–7.83) for three mutations relative to control participants, and ORs for high daily intake of B[a]Ps from meat were 1.17 (95% CI, 0.79–1.74) for one mutation, 1.79 (95% CI, 0.64–5.04) for two mutations, and 8.04 (95% CI, 2.29–28.27) for three mutations.
Table 5.
Associations between PAH-related exposures and the number of tumor p53 mutations relative to control participants in the LIBCSP.a
OR (95% CI) |
|||
---|---|---|---|
No. of mutations | Cases/controls (n) | Age adjusted | Multivariate adjusted |
PAH–DNA adducts (detectable vs. nondetectable) | |||
1 | 55/941 | 1.06 (0.58–1.94) | 1.19 (0.63–2.25) |
2 | 10/941 | 1.85 (0.38–9.01) | 1.87 (0.38–9.20) |
3 | 15/941 | 2.10 (0.58–7.58) | 2.15 (0.59–7.83) |
Ever active smoking vs. never active smoking | |||
1 | 113/1,556 | 0.89 (0.61–1.32) | 0.94 (0.63–1.40) |
2 | 16/1,556 | 0.84 (0.31–2.28) | 0.98 (0.35–2.72) |
3 | 18/1,556 | 0.96 (0.38–2.46) | 1.13 (0.44–2.92) |
Current active smoking vs. never active smoking | |||
1 | 72/989 | 0.83 (0.47–1.47) | 0.90 (0.51–1.62) |
2 | 10/989 | 0.83 (0.16–4.23) | 0.88 (0.17–4.57) |
3 | 9/989 | — | — |
Past active smoking vs. never active smoking | |||
1 | 96/1,262 | 0.93 (0.61–1.43) | 0.99 (0.64–1.52) |
2 | 14/1,262 | 0.96 (0.32–2.86) | 1.08 (0.36–3.30) |
3 | 18/1,262 | 1.36 (0.53–3.50) | 1.60 (0.61–4.18) |
Both active and passive smoking vs. never passive or active smoking | |||
1 | 60/875 | 0.65 (0.36–1.17) | 0.69 (0.37–1.27) |
2 | 8/875 | 0.72 (0.14–3.71) | 0.87 (0.17–4.61) |
3 | 9/875 | — | — |
Active smoking only vs. never passive or active smoking | |||
1 | 33/328 | 1.14 (0.53–2.42) | 1.23 (0.57–2.66) |
2 | 4/328 | 1.39 (0.19–10.31) | 1.50 (0.20–11.38) |
3 | 0/328 | — | — |
Ever passive smoking only vs. never passive or active smoking | |||
1 | 54/681 | 0.78 (0.42–1.42) | 0.81 (0.44–1.49) |
2 | 8/681 | 1.71 (0.32–9.21) | 1.73 (0.32–9.38) |
3 | 9/681 | — | — |
Ever passively exposed to spouse vs. never passively exposed to spouse | |||
1 | 80/1,228 | 1.50 (0.92–2.46) | 1.51 (0.92–2.46) |
2 | 12/1,228 | 2.15 (0.61–7.56) | 2.21 (0.63–7.70) |
3 | 18/1,228 | 3.36 (0.94–12.04) | 3.23 (0.90–11.57) |
Lifetime intake of smoked/grilled meat (high vs. low)b | |||
1 | 110/1,475 | 0.98 (0.66–1.46) | 0.98 (0.66–1.46) |
2 | 16/1,475 | 3.64 (1.12–11.79) | 3.64 (1.12–11.79) |
3 | 18/1,475 | 1.16 (0.45–2.99) | 1.16 (0.45–2.99) |
Total B[a]Ps from meat (high intake vs. low intake)c | |||
1 | 109/1,475 | 1.17 (0.79–1.74) | 1.17 (0.79–1.74) |
2 | 16/1,475 | 1.79 (0.64–5.04) | 1.79 (0.64–5.04) |
3 | 18/1,475 | 8.04 (2.29–28.27) | 8.04 (2.29–28.27) |
—, insufficient sample size.
In addition to adjustment for age group, final models were adjusted for daily alcohol intake when examining smoking exposure and age at menarche when examining PAH–DNA adducts.
Lifetime intake of grilled and smoked meat is dichotomized based on median lifetime servings among controls (median, 4,160 servings).
Daily intake of B[a]Ps from meat is dichotomized based on median daily intake among controls (median, 0.42 ng/day).
We also examined associations of p53 mutation status with active smoking and lifetime intake of grilled and smoked meat using referent groups consisting of never smokers with low intake of grilled and smoked meat. Use of this approach strengthened associations between PAH-related factors and p53 mutation–negative cancer, whereas associations with p53 mutation–positive cancer were essentially unchanged [see Supplemental Material, Table 1 (doi:10.1289/ehp.0901233)]. In these analyses, p53 mutation–negative cancer was associated with smoking history (ever vs. never; OR = 1.31; 95% CI, 1.03–1.67), current smoking (OR = 1.43; 95% CI, 1.06–1.93), and lifetime intake of grilled and smoked meat (OR = 1.61; 95% CI, 1.27–2.05).
Relations between PAH-related exposures and G:C→A:T transitions at CpG sites, insertions/deletions, and frameshift mutations were also strengthened by using the alternative referent groups. For example, examining associations between current smoking and insertions/deletions and between grilled and smoked meat intake and G:C→A:T transitions at CpG sites yielded ORs of 3.06 (95% CI, 0.87–10.77) and 2.68 (95% CI, 0.89–8.09), respectively [see Supplemental Material, Table 2 (doi:10.1289/ehp.0901233)]. We did not examine mutation number, A:T→G:C transitions, or G:C→T:A transversions due to low numbers of subjects with these mutations. Results were not altered substantially for missense, nonsense, and silent mutations (data not shown). Comparing current smokers who had high lifetime intake of grilled and smoked meat with never smokers who had low intake of grilled and smoked meat yielded ORs of 1.53 (95% CI, 1.07–2.20) for p53 mutation–negative cancer, 4.24 (95% CI, 1.00–17.94) for G:C→A:T transitions at CpG sites, 4.49 (95% CI, 1.05–19.25) for insertions/deletions, and 4.43 (95% CI, 1.04–18.98) for frameshift mutations.
Discussion
In this population-based analysis, we found that participants with breast tumor p53 mutations were less likely to be exposed to PAH-related sources than were participants with p53 mutation–negative cancer. However, frameshift mutations and number of mutations were consistently elevated in exposed subjects, and tumors of women exposed to PAH-related sources showed a pattern of increased G:C→A:T transitions at CpG sites and insertions/deletions. Associations of PAH-related exposures with p53 mutation status, type, and effect were strengthened by minimizing PAH exposure in referent groups.
This is the first study to examine associations of dietary PAH intake, PAH–DNA adducts, and passive smoking with breast tumor p53 mutations. It is the third study to examine associations between active smoking and breast cancer p53 mutations, and has a larger sample size than the previous investigations (Conway et al. 2002; Van Emburgh et al. 2008). Few studies have looked at relations between exogenous exposures and p53 mutations in breast cancer, although such research has potential to provide insights regarding breast cancer etiology.
We found a relatively low prevalence of p53 mutations (15%) among our participants, which is consistent with the wide range reported in the literature (11–35%) (Goldman and Shields 1998; Tennis et al. 2006; Van Emburgh et al. 2008). This variation across studies may be due to differences between study populations, such as differences in distribution of age and race (Bowen et al. 2006; Klauber-DeMore 2005). Methodologic errors in mutation detection may also have contributed to the modest mutation prevalence. However, we selected a method previously shown to have a high sensitivity (Qiu et al. 2004) and that has been used successfully in various applications, including detection of p53 mutations in hematologic malignancies (Mitani et al. 2007).
Immunohistochemical staining estimates p53 protein expression and is widely used as a proxy measure for detection of p53 mutation status. However, the sensitivity of this method relative to mutation analysis is < 75% for breast cancer (Lacroix et al. 2006), and immunohistochemistry is subject to a number of methodologic limitations (Hall and McCluggage 2006; McCabe et al. 2005). We detected overexpression in 36% of tumor samples (Rossner et al. 2008), which is consistent with the range reported in the literature (30–40%) (Erdem et al. 2005; Iwase et al. 2001), but we did not find evidence of heterogeneity in the ORs for the associations between PAH-related exposures and p53-positive cancer as defined by protein expression status and the corresponding PAH exposures and p53-negative breast cancer. This is consistent with the results of one study of smoking and p53 overexpression (Furberg et al. 2002), and inconsistent with two other studies that noted an association between smoking and p53-positive breast cancer among younger women (Gammon et al. 1999; van der Kooy et al. 1996). Potential explanations for the discrepant findings across investigations include inability to identify specific p53 mutational subtypes when using immunohistochemistry as a proxy, differences in metabolic activation and detoxification of PAHs between study populations, and chance findings.
Conway et al. (2002) found that current smokers were more likely and former smokers were less likely than never smokers to have p53 mutation–positive breast cancer. In contrast, we found that both current and former smokers were less likely than never smokers to have p53 mutation–positive cancer. Another epidemiologic study found positive, nonsignificant associations between smoking history and p53 mutation prevalence (Van Emburgh et al. 2008). However, the number of p53 mutation–positive cases (n = 34, mutation prevalence = 11%) was substantially smaller than in our study (n = 128, mutation prevalence = 15%) or in the study by Conway et al. (2002; n = 108, mutation prevalence = 24%), and the results appeared to be unstable. Reasons potentially underlying inconsistent results between studies include differences in age and race distributions and in metabolism and detoxification of PAHs between study populations, varying definitions of current smoking status, methodologic differences in mutation analysis, and chance findings.
The elevated associations between PAH-related exposures and p53 mutation–negative cancer may indicate that PAH-related factors are related to breast cancer through mechanisms other than p53 mutation. Grilled and smoked meat and tobacco smoke contain carcinogens other than PAHs, and PAH–DNA adducts or increased oxidative stress may lead to mutations in genes other than p53. Induction of DNA repair could also contribute to decreased mutation levels among women exposed to PAHs (Wei et al. 2000). In vitro and in vivo investigations indicate that repair is important in determining mutation patterns (Greenblatt et al. 1994). Furthermore, the fact that p53 mutation patterns in tobacco-associated cancers show surprising variation is thought to be due at least partly to differences in DNA repair between cancer sites (Greenblatt et al. 1994). We found evidence of statistical heterogeneity in the ORs between p53 mutation–positive and p53 mutation–negative cancer when looking at exposure to both active and passive smoking. Associations between other PAH-related exposures and breast cancer did not differ statistically between mutation status subtypes, possibly due to insufficient power to detect such differences. Inverse associations between PAH exposures and p53 mutation–positive cancer may be due to random variation around the null.
PAH-related exposures have been shown to increase both frameshift and base substitution mutations (Adonis and Gil 2000), and specific mutation effects may have etiologic associations. Relations of PAH exposures with nonsense and silent mutations were inconsistent in our study. Results for p53 missense mutations were inconsistent as well, despite a larger sample size, with smoking and detectable adducts showing inverse associations and dietary PAH intake showing a positive association with missense mutations. It is plausible that different PAH-related exposures could lead to differing mutation effects, although this inconsistency may also be due to chance. Frameshift mutations were consistently elevated in exposed subjects, especially when looking at adducts and a combined measure of smoking and intake of grilled and smoked meat. PAHs induce frameshift mutations through adduct-induced deformation of the DNA helix (Greenblatt et al. 1994).
Participants with PAH-related exposures exhibited a fairly consistent mutational spectrum, characterized by increased proportions of insertions/deletions and G:C→A:T transitions at CpG sites. We found inconsistent results regarding G:C→A:T transversions and G:C→A:T transitions at non-CpG sites. This is in contrast to a previous study that reported that smokers showed an increased proportion of breast tumor G:C→T:A transversions and found some suggestion of decreased G:C→A:T transitions at CpG sites (Conway et al. 2002).
Previous research has suggested that the p53 mutational spectrum of breast cancer includes high proportions of G:C→T:A transversions, G:C→A:T transitions at CpG sites, and insertions/deletions (Biggs et al. 1993; Goldman and Shields 1998; Greenblatt et al. 1994). The latter two mutation types are thought to result from endogenous processes (Greenblatt et al. 1994). However, it is possible that certain carcinogens produce a mutational spectrum similar to that due to endogenous processes (Biggs et al. 1993). For example, although benzo[a]pyrene diol epoxide adducts have been strongly associated with G→T transversions in vitro (Eisenstadt et al. 1982; Ruggeri et al. 1993), G→A transitions occur as the predominant mutation in vivo in some contexts because of influences of the local environment (Shukla et al. 1997). PAHs have been associated with transitions at G:C base pairs (Harris 1991), and transitions and frameshifts may be induced by PAH–DNA adducts (Greenblatt et al. 1994). PAHs may also cause DNA damage by generating reactive oxygen species, an endogenous mutagen (Singh et al. 2007). Moreover, it is very plausible that some carcinogens influence the rate of accumulation of mutations without altering the pattern (Biggs et al. 1993). The latter hypothesis is supported by our finding that likelihood of PAH exposure increases with tumor p53 mutation number.
A number of studies found results similar to ours when examining associations between PAH-related sources and p53 mutations in smoking-related cancers (Diergaarde et al. 2003; Fryzek et al. 2006; Harty et al. 1996; Schroeder et al. 2003; Zhang et al. 2006). Most studies that examined p53 mutational spectra found a difference in spectrum by exposure status, despite null or inverse associations with p53 mutation prevalence, possibly because associations with specific mutation patterns were washed out when all mutations were combined into a single case subgroup. For example, a study by Schroeder et al. (2003) that observed no difference in p53 mutation frequency in bladder cancer according to smoking status found that smoking was strongly associated with CpG G:C→A:T transitions.
The main limitation of our study is the sample size for examining subgroup mutation effects, for example, by type or number. Some of our point estimates have very wide CI estimates, and these results should be interpreted with caution. We cannot rule out that our findings are due to chance. However, this is the largest study regarding PAH-related exposures and breast tumor p53 mutations conducted to date, and the first study to look at associations for most of the PAH-related exposures examined in this investigation. Thus, we believe that our analysis is an important addition to the sparse literature for this topic. The strengthened associations observed after minimizing PAH exposure in referent groups provide further support for a relation between PAHs and breast cancer p53 mutation status, type, and effect.
A potential limitation in any retrospective, case–control analysis is the possibility of recall bias. However, cases were unaware of the mutation patterns in their tumor tissue, so this potential bias is less likely to affect case–case comparisons. Many of the exposure variables examined were surrogates of PAH exposure, although PAH–DNA adducts are an internal measure of PAH exposure and response (Gammon and Santella 2008). However, PAH–DNA adducts reflect only recent exposures, whereas exposures in the more distant past are likely to be relevant to carcinogenesis. Evaluation of exons 5–8 only is likely to underestimate the prevalence of p53 mutations. However, these exons contain > 90% of mutations reported in breast cancer (Lacroix et al. 2006). Missense mutations are concentrated in the central part of p53, whereas nonsense, silent, and frameshift mutations are distributed throughout the coding region (Greenblatt et al. 1994).
Previous research has suggested that associations between PAHs and p53 mutation pattern may vary by genetic variants for detoxification and DNA repair enzymes (Biggs et al. 1993; Schroeder et al. 2003; Van Emburgh et al. 2008) and that the carcinogenic effects of PAHs on the breast may be stronger among women with low antioxidant intake (Steck et al. 2007). Therefore, future high-powered analyses should examine effect modification by genotypes relevant to detoxification, antioxidative response, and DNA repair and by antioxidant intake. Future studies should also categorize exposures more finely and should assess the importance of timing of PAH exposure on p53 mutagenesis.
Conclusions
Our findings suggest that PAH exposures may be associated with breast tumor p53 mutation effect, type, and number rather than with overall p53 mutations, and may also be related to breast cancer through mechanisms other than p53 mutation. The high incidence of breast cancer implies that even modestly increased risks for tumor subgroups may have substantial public health significance. This analysis has extended previous research regarding a sparsely investigated topic. Our results provide new information to guide future research regarding the carcinogenic effects of PAH exposure on the human breast.
Footnotes
This work was supported in part by grants U01 CA/ES66572, P30ES009089, P30ES10126, and T32-CA09330 from the National Cancer Institute and the National Institute of Environmental Health Sciences; awards from the U.S. Army (BC972772), Breast Cancer Research Foundation and Women at Risk Program; and gifts from private citizens.
Supplemental Material is available online (doi:10.1289/ehp.0901233 via http://dx.doi.org/).
S.E. was employed at Pfizer, Inc., during the analysis phase of the manuscript; the company did not participate in the design, conduct, interpretation, or publication of this study. The authors declare they have no actual or potential competing financial or nonfinancial interests.
References
- Adonis M, Gil L. Polycyclic aromatic hydrocarbon levels and mutagenicity of inhalable particulate matter in Santiago, Chile. Inhal Toxicol. 2000;12:1173–1183. doi: 10.1080/08958370050198520. [DOI] [PubMed] [Google Scholar]
- Ambrosone CB, Kropp S, Yang J, Yao S, Shields PG, Chang-Claude J. Cigarette smoking, N-acetyltransferase 2 genotypes, and breast cancer risk: pooled analysis and meta-analysis. Cancer Epidemiol Biomarkers Prev. 2008;17:15–26. doi: 10.1158/1055-9965.EPI-07-0598. [DOI] [PubMed] [Google Scholar]
- American Cancer Society. Cancer Facts and Figures. Atlanta, GA: American Cancer Society; 2008. [Google Scholar]
- Besaratinia A, Kleinjans JC, Van Schooten FJ. Biomonitoring of tobacco smoke carcinogenicity by dosimetry of DNA adducts and genotyping and phenotyping of biotransformational enzymes: a review on polycyclic aromatic hydrocarbons. Biomarkers. 2002;7:209–229. doi: 10.1080/13547500110120000. [DOI] [PubMed] [Google Scholar]
- Biggs PJ, Warren W, Venitt S, Stratton MR. Does a genotoxic carcinogen contribute to human breast cancer? The value of mutational spectra in unraveling the aetiology of cancer. Mutagenesis. 1993;8:275–283. doi: 10.1093/mutage/8.4.275. [DOI] [PubMed] [Google Scholar]
- Block G, Hartman AM, Dresser CM, Carroll MD, Gannon J, Gardner L. A data-based approach to diet questionnaire design and testing. Am J Epidemiol. 1986;124:453–469. doi: 10.1093/oxfordjournals.aje.a114416. [DOI] [PubMed] [Google Scholar]
- Bonner MR, Han D, Nie J, Rogerson P, Vena JE, Muti P, et al. Breast cancer risk and exposure in early life to polycyclic aromatic hydrocarbons using total suspended particulates as a proxy measure. Cancer Epidemiol Biomarkers Prev. 2005;14:53–60. [PubMed] [Google Scholar]
- Bowen RL, Stebbing J, Jones LJ. A review of the ethnic differences in breast cancer. Pharmacogenomics. 2006;7:935–942. doi: 10.2217/14622416.7.6.935. [DOI] [PubMed] [Google Scholar]
- Braithwaite E, Wu X, Wang Z. Repair of DNA lesions: mechanisms and relative repair efficiencies. Mutat Res. 1999;424:207–219. doi: 10.1016/s0027-5107(99)00020-2. [DOI] [PubMed] [Google Scholar]
- Conway K, Edmiston SN, Cui L, Drouin SS, Pang J, He M, et al. Prevalence and spectrum of p53 mutations associated with smoking in breast cancer. Cancer Res. 2002;62:1987–1995. [PubMed] [Google Scholar]
- Diergaarde B, Vrieling A, van Kraats AA, van Muijen GN, Kok FJ, Kampman E. Cigarette smoking and genetic alterations in sporadic colon carcinomas. Carcinogenesis. 2003;24:565–571. doi: 10.1093/carcin/24.3.565. [DOI] [PubMed] [Google Scholar]
- Eisenstadt E, Warren AJ, Porter J, Atkins D, Miller JH. Carcinogenic epoxides of benzo[a]pyrene and cyclopenta[cd]pyrene induce base substitutions via specific transversions. Proc Natl Acad Sci USA. 1982;79:1945–1949. doi: 10.1073/pnas.79.6.1945. [DOI] [PMC free article] [PubMed] [Google Scholar]
- el-Bayoumy K, Chae YH, Upadhyaya P, Rivenson A, Kurtzke C, Reddy B, et al. Comparative tumorigenicity of benzo[a]pyrene, 1-nitropyrene and 2-amino-1-methyl-6-phenylimidazo[4,5-b]pyridine administered by gavage to female CD rats. Carcinogenesis. 1995;16:431–434. doi: 10.1093/carcin/16.2.431. [DOI] [PubMed] [Google Scholar]
- Erdem O, Dursun A, Coskun U, Gunel N. The prognostic value of p53 and cerB2 expression, proliferative activity and angiogenesis in node-negative breast carcinoma. Tumori. 2005;91:46–52. doi: 10.1177/030089160509100109. [DOI] [PubMed] [Google Scholar]
- Fryzek JP, Garabrant DH, Schenk M, Kinnard M, Greenson JK, Sarkar FH. The association between selected risk factors for pancreatic cancer and the expression of p53 and K-ras codon 12 mutations. Int J Gastrointest Cancer. 2006;37:139–145. doi: 10.1007/s12029-007-9005-8. [DOI] [PubMed] [Google Scholar]
- Furberg H, Millikan RC, Geradts J, Gammon MD, Dressler LG, Ambrosone CB, et al. Environmental factors in relation to breast cancer characterized by p53 protein expression. Cancer Epidemiol Biomarkers Prev. 2002;11:829–835. [PubMed] [Google Scholar]
- Gammon MD, Eng SM, Teitelbaum SL, Britton JA, Kabat GC, Hatch M, et al. Environmental tobacco smoke and breast cancer incidence. Environ Res. 2004a;96:176–185. doi: 10.1016/j.envres.2003.08.009. [DOI] [PubMed] [Google Scholar]
- Gammon MD, Hibshoosh H, Terry MB, Bose S, Schoenberg JB, Brinton LA, et al. Cigarette smoking and other risk factors in relation to p53 expression in breast cancer among young women. Cancer Epidemiol Biomarkers Prev. 1999;8:255–263. [PubMed] [Google Scholar]
- Gammon MD, Neugut AI, Santella RM, Teitelbaum SL, Britton JA, Terry MB, et al. The Long Island Breast Cancer Study Project: description of a multi-institutional collaboration to identify environmental risk factors for breast cancer. Breast Cancer Res Treat. 2002a;74:235–254. doi: 10.1023/a:1016387020854. [DOI] [PubMed] [Google Scholar]
- Gammon MD, Sagiv SK, Eng SM, Shantakumar S, Gaudet MM, Teitelbaum SL, et al. Polycyclic aromatic hydrocarbon-DNA adducts and breast cancer: a pooled analysis. Arch Environ Health. 2004b;59:640–649. doi: 10.1080/00039890409602948. [DOI] [PMC free article] [PubMed] [Google Scholar]
- Gammon MD, Santella RM. PAH, genetic susceptibility and breast cancer risk: an update from the Long Island Breast Cancer Study Project. Eur J Cancer. 2008;44:636–640. doi: 10.1016/j.ejca.2008.01.026. [DOI] [PubMed] [Google Scholar]
- Gammon MD, Santella RM, Neugut AI, Eng SM, Teitelbaum SL, Paykin A, et al. Environmental toxins and breast cancer on Long Island. I. Polycyclic aromatic hydrocarbon DNA adducts. Cancer Epidemiol Biomarkers Prev. 2002b;11:677–685. [PubMed] [Google Scholar]
- Goldman R, Shields PG. Molecular epidemiology of breast cancer. In Vivo. 1998;12:43–48. [PubMed] [Google Scholar]
- Greenblatt MS, Bennett WP, Hollstein M, Harris CC. Mutations in the p53 tumor suppressor gene: clues to cancer etiology and molecular pathogenesis. Cancer Res. 1994;54:4855–4878. [PubMed] [Google Scholar]
- Hall PA, McCluggage WG. Assessing p53 in clinical contexts: unlearned lessons and new perspectives. J Pathol. 2006;208:1–6. doi: 10.1002/path.1913. [DOI] [PubMed] [Google Scholar]
- Harris CC. Chemical and physical carcinogenesis: advances and perspective for the 1990s. Cancer Res. 1991;51:5023s–5044s. [PubMed] [Google Scholar]
- Harty LC, Guinee DG, Jr, Travis WD, Bennett WP, Jett J, Colby TV, et al. p53 mutations and occupational exposures in a surgical series of lung cancers. Cancer Epidemiol Biomarkers Prev. 1996;5:997–1003. [PubMed] [Google Scholar]
- Hecht SS. Tobacco smoke carcinogens and breast cancer. Environ Mol Mutagen. 2002;39:119–126. doi: 10.1002/em.10071. [DOI] [PubMed] [Google Scholar]
- Holmes MD, Colditz GA, Hunter DJ, Hankinson SE, Rosner B, Speizer FE, et al. Meat, fish and egg intake and risk of breast cancer. Int J Cancer. 2003;104:221–227. doi: 10.1002/ijc.10910. [DOI] [PubMed] [Google Scholar]
- Hosmer D, Lemeshow S. Applied Logistic Regression. New York: John Wiley & Sons; 1989. [Google Scholar]
- Iwase H, Ando Y, Ichihara S, Toyoshima S, Nakamura T, Karamatsu S, et al. Immunohistochemical analysis on biological markers in ductal carcinoma in situ of the breast. Breast Cancer. 2001;8:98–104. doi: 10.1007/BF02967487. [DOI] [PubMed] [Google Scholar]
- Kazerouni N, Sinha R, Hsu CH, Greenberg A, Rothman N. Analysis of 200 food items for benzo[a]pyrene and estimation of its intake in an epidemiologic study. Food Chem Toxicol. 2001;39:423–436. doi: 10.1016/s0278-6915(00)00158-7. [DOI] [PubMed] [Google Scholar]
- Klauber-Demore N. Tumor biology of breast cancer in young women. Breast Dis. 2005;23:9–15. doi: 10.3233/bd-2006-23103. [DOI] [PubMed] [Google Scholar]
- Lacroix M, Toillon RA, Leclercq G. p53 and breast cancer, an update. Endocr Relat Cancer. 2006;13:293–325. doi: 10.1677/erc.1.01172. [DOI] [PubMed] [Google Scholar]
- Levine AJ. p53, the cellular gatekeeper for growth and division. Cell. 1997;88:323–331. doi: 10.1016/s0092-8674(00)81871-1. [DOI] [PubMed] [Google Scholar]
- Lewis RG, Fortune CR, Willis RD, Camann DE, Antley JT. Distribution of pesticides and polycyclic aromatic hydrocarbons in house dust as a function of particle size. Environ Health Perspect. 1999;107:721–726. doi: 10.1289/ehp.99107721. [DOI] [PMC free article] [PubMed] [Google Scholar]
- Lioy PJ, Greenberg A. Factors associated with human exposures to polycyclic aromatic hydrocarbons. Toxicol Ind Health. 1990;6:209–223. [PubMed] [Google Scholar]
- McCabe A, Dolled-Filhart M, Camp RL, Rimm DL. Automated quantitative analysis (AQUA) of in situ protein expression, antibody concentration, and prognosis. J Natl Cancer Inst. 2005;97:1808–1815. doi: 10.1093/jnci/dji427. [DOI] [PubMed] [Google Scholar]
- Mitani N, Niwa Y, Okamoto Y. Surveyor nuclease-based detection of p53 gene mutations in haematological malignancy. Ann Clin Biochem. 2007;44:557–559. doi: 10.1258/000456307782268174. [DOI] [PubMed] [Google Scholar]
- Phillips DH. Polycyclic aromatic hydrocarbons in the diet. Mutat Res. 1999;443:139–147. doi: 10.1016/s1383-5742(99)00016-2. [DOI] [PubMed] [Google Scholar]
- Qiu P, Shandilya H, D’Alessio J, O’Connor K, Durocher J, Gerard G. Mutation detection using Surveyor nuclease. Biotechniques. 2004;36:702–707. doi: 10.2144/04364PF01. [DOI] [PubMed] [Google Scholar]
- Rossner P, Gammon M, Zhang Y, Terry M, Hibshoosh H, Memeo L, et al. Mutations in p53, p53 protein overexpression and breast cancer survival. J Cell Mol Med. 2008 doi: 10.1111/j.158. [DOI] [PMC free article] [PubMed] [Google Scholar]
- Ruggeri B, DiRado M, Zhang SY, Bauer B, Goodrow T, Klein-Szanto AJ. Benzo[a]pyrene-induced murine skin tumor exhibit frequent and characteristic G to T mutations in the p53 gene. Proc Natl Acad Sci USA. 1993;90:1013–1017. doi: 10.1073/pnas.90.3.1013. [DOI] [PMC free article] [PubMed] [Google Scholar]
- Rundle A, Tang D, Hibshoosh H, Estabrook A, Schnabel F, Cao W, et al. The relationship between genetic damage from polycyclic aromatic hydrocarbons in breast tissue and breast cancer. Carcinogenesis. 2000;21:1281–1289. [PubMed] [Google Scholar]
- Russo J, Tahin Q, Lareef MH, Hu YF, Russo IH. Neoplastic transformation of human breast epithelial cells by estrogens and chemical carcinogens. Environ Mol Mutagen. 2002;39:254–263. doi: 10.1002/em.10052. [DOI] [PubMed] [Google Scholar]
- Samanta SK, Singh OV, Jain RK. Polycyclic aromatic hydrocarbons: environmental pollution and bioremediation. Trends Biotechnol. 2002;20:243–248. doi: 10.1016/s0167-7799(02)01943-1. [DOI] [PubMed] [Google Scholar]
- Santella RM. Immunological methods for detection of carcinogen-DNA damage in humans. Cancer Epidemiol Biomarkers Prev. 1999;8:733–739. [PubMed] [Google Scholar]
- Santodonato J. Review of the estrogenic and antiestrogenic activity of polycyclic aromatic hydrocarbons: relationship to carcinogenicity. Chemosphere. 1997;34:835–848. doi: 10.1016/s0045-6535(97)00012-x. [DOI] [PubMed] [Google Scholar]
- Schlesselman JJ. Case-Control Studies. New York: Oxford University Press; 1982. [Google Scholar]
- Schroeder JC, Conway K, Li Y, Mistry K, Bell DA, Taylor JA. p53 mutations in bladder cancer: evidence for exogenous versus endogenous risk factors. Cancer Res. 2003;63:7530–7538. [PubMed] [Google Scholar]
- Shantakumar S, Gammon MD, Eng SM, Sagiv SK, Gaudet MM, Teitelbaum SL, et al. Residential environmental exposures and other characteristics associated with detectable PAH-DNA adducts in peripheral mononuclear cells in a population-based sample of adult females. J Expo Anal Environ Epidemiol. 2005;15:482–490. doi: 10.1038/sj.jea.7500426. [DOI] [PubMed] [Google Scholar]
- Shrier I, Platt RW. Reducing bias through directed acyclic graphs. BMC Med Res Methodol. 2008;8:70. doi: 10.1186/1471-2288-8-70. [Online 30 October 2008] [DOI] [PMC free article] [PubMed] [Google Scholar]
- Shukla R, Liu T, Geacintov NE, Loechler EL. The major, N2-dG adduct of (+)-anti-B[a]PDE shows a dramatically different mutagenic specificity (predominantly, G → A) in a 5′-CGT-3′ sequence context. Biochemistry. 1997;36:10256–10261. doi: 10.1021/bi970541+. [DOI] [PubMed] [Google Scholar]
- Singh R, Kaur B, Kalina I, Popov TA, Georgieva T, Garte S, et al. Effects of environmental air pollution on endogenous oxidative DNA damage in humans. Mutat Res. 2007;620:71–82. doi: 10.1016/j.mrfmmm.2007.02.024. [DOI] [PubMed] [Google Scholar]
- Steck SE, Gaudet MM, Eng SM, Britton JA, Teitelbaum SL, Neugut AI, et al. Cooked meat and risk of breast cancer—lifetime versus recent dietary intake. Epidemiology. 2007;18:373–382. doi: 10.1097/01.ede.0000259968.11151.06. [DOI] [PubMed] [Google Scholar]
- Tennis M, Krishnan S, Bonner M, Ambrosone CB, Vena JE, Moysich K, et al. p53 mutation analysis in breast tumors by a DNA microarray method. Cancer Epidemiol Biomarkers Prev. 2006;15:80–85. doi: 10.1158/1055-9965.EPI-05-0444. [DOI] [PubMed] [Google Scholar]
- Terry PD, Goodman M. Is the association between cigarette smoking and breast cancer modified by genotype? A review of epidemiologic studies and meta-analysis. Cancer Epidemiol Biomarkers Prev. 2006;15:602–611. doi: 10.1158/1055-9965.EPI-05-0853. [DOI] [PubMed] [Google Scholar]
- Terry PD, Rohan TE. Cigarette smoking and the risk of breast cancer in women: a review of the literature. Cancer Epidemiol Biomarkers Prev. 2002;11:953–971. [PubMed] [Google Scholar]
- van der Kooy K, Rookus MA, Peterse HL, Van Leeuwen FE. p53 protein overexpression in relation to risk factors for breast cancer. Am J Epidemiol. 1996;144:924–933. doi: 10.1093/oxfordjournals.aje.a008862. [DOI] [PubMed] [Google Scholar]
- Van Emburgh BO, Hu JJ, Levine EA, Mosley LJ, Case LD, Lin HY, et al. Polymorphisms in drug metabolism genes, smoking, and p53 mutations in breast cancer. Mol Carcinog. 2008;47:88–99. doi: 10.1002/mc.20365. [DOI] [PMC free article] [PubMed] [Google Scholar]
- Wei Q, Cheng L, Amos CI, Wang LE, Guo Z, Hong WK, et al. Repair of tobacco carcinogen-induced DNA adducts and lung cancer risk: a molecular epidemiologic study. J Natl Cancer Inst. 2000;92:1764–1772. doi: 10.1093/jnci/92.21.1764. [DOI] [PubMed] [Google Scholar]
- Zhang YJ, Rossner P, Jr, Chen Y, Agrawal M, Wang Q, Wang L, et al. Aflatoxin B1 and polycyclic aromatic hydrocarbon adducts, p53 mutations and p16 methylation in liver tissue and plasma of hepatocellular carcinoma patients. Int J Cancer. 2006;119:985–991. doi: 10.1002/ijc.21699. [DOI] [PubMed] [Google Scholar]
- Zheng W, Gustafson DR, Sinha R, Cerhan JR, Moore D, Hong CP, et al. Well-done meat intake and the risk of breast cancer. J Natl Cancer Inst. 1998;90:1724–1729. doi: 10.1093/jnci/90.22.1724. [DOI] [PubMed] [Google Scholar]