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BMC Cancer logoLink to BMC Cancer
. 2006 Jun 29;6:173. doi: 10.1186/1471-2407-6-173

Polymorphisms in estrogen-metabolizing and estrogen receptor genes and the risk of developing breast cancer among a cohort of women with benign breast disease

Lisa Gallicchio 1,2,, Sonja I Berndt 1, Meghan A McSorley 1, Craig J Newschaffer 1, Lucy W Thuita 1, Pedram Argani 3, Sandra C Hoffman 1, Kathy J Helzlsouer 1,2
PMCID: PMC1534058  PMID: 16808847

Abstract

Background

A cohort study was conducted to examine the role of genetic polymorphisms in three estrogen metabolizing enzymes (COMT, CYP1A1, CYP1B1) and the two estrogen receptors (ESR1, ESR2) in the progression of benign breast disease (BBD) to breast cancer.

Methods

Among participants in an ongoing cohort study, 1438 Caucasian women had a breast biopsy for BBD and were successfully genotyped for at least one of the polymorphisms examined in this study. Genotypes were determined using DNA extracted from blood specimens collected in 1989. Incident cases of breast cancer occurring subsequent to BBD diagnosis up to 2003 were identified through cancer registries.

Results

Among all participants, the ESR2 *5772G allele was associated with a significant decrease in the risk of breast cancer among women with BBD (Odds Ratio (OR) 0.38; 95% Confidence Interval (CI) 0.15, 0.96). Compared to the reference wild-type genotypes, marginally significant associations with the development of breast cancer were observed between carriers of the variant ESR1 – 104062T allele (OR 0.70, 95% CI 0.45, 1.09), the variant ESR2 *38A allele (OR 1.40; 95% CI 0.88, 2.25), and the variant CYP1B1 453Ser allele (OR 1.48, 95% CI 0.95, 2.32).

Conclusion

The results indicate that specific polymorphisms in the CYP1B1, ESR1, and ESR2 genes may play a role in progression of BBD to breast cancer among Caucasian women. Although additional studies are needed to confirm or refute our findings, these results suggest that genetic markers may aid in the identification of women who are at risk for progression of BBD to cancer.

Background

Biopsy-proven benign breast disease (BBD) is a well-defined risk factor for developing invasive breast cancer [1,2]. However, little is known about which women with BBD progress to have a subsequent in situ or invasive cancer. A woman's level of endogenous estrogen may be important in the progression of BBD to invasive breast cancer. Abundant evidence suggests that estrogen is an important factor in the development of breast cancer among average-risk women. This evidence includes findings from recent prospective studies that showed significantly increased levels of serum estrogen in women who developed breast cancer compared to women who did not develop breast cancer [3-7]. In addition, numerous studies have reported that risk factors associated with prolonged estrogen exposure, such as early age at menarche, nulliparity, and older age at first birth, increase a woman's risk of developing breast cancer (reviewed by Mitrunen and Hirvonen [8]).

Because of the importance of estrogen in the development of breast cancer among average-risk women, it is plausible that polymorphisms in estrogen metabolizing genes may be associated with the risk of developing breast cancer among women with BBD. Estrogens undergo oxidative metabolism by several cytochrome P450 (CYPs) enzymes [9]; the major metabolic pathways are 2-hydroxylation, which is primarily catalyzed by CYP1A1, and 4-hydroxylation, which is dominated by CYP1B1 [10]. The hydroxylated estrogens are then either converted to semiquinones or quinones, which can produce DNA adducts and lead to oxidative damage to lipids and DNA, or inactivated by catechol O-methyltransferase (COMT) [10-13]. Within the genes encoding for CYP1A1, CYP1B1, and COMT, a number of polymorphisms have been identified, some which have been shown in laboratory studies to be functional (8). The associations of some of these polymorphisms with the risk of developing breast cancer among average risk women have been studied, and most of the findings have been inconsistent (reviewed in Mitrunen and Hirvonen [8]). No study has examined the associations of polymorphisms in CYP1A1, CYP1B1, and COMT with breast cancer risk among women with BBD.

While the estrogen metabolizing enzymes may influence the levels of circulating endogenous estrogens and, therefore, contribute to breast cancer risk, the estrogen receptors determine, in part, the action of estrogens on the mammary gland. Estrogen acts on target tissues by binding to the estrogen receptors, which exist in two forms, ER-α or ESR1 and ER-β or ESR2 [14,15]. Like the estrogen metabolizing enzymes, a number of polymorphisms in both ER genes have been identified [16], and it has been hypothesized that these polymorphisms may increase or decrease a woman's breast cancer risk depending on the functional consequence of the polymorphism. Several studies have investigated the associations between polymorphisms in the ESR1 and ESR2 genes and the risk of breast cancer among average-risk women and have reported mixed results [16-29]. To our knowledge, however, no study has examined the associations of polymorphisms in ESR1 and ESR2 with breast cancer risk among women with BBD.

The aim of the present study was to analyze the associations between genetic polymorphisms in three estrogen metabolizing enzymes (COMT, CYP1A1, CYP1B1) and the two estrogen receptors (ESR1, ESR2) and the risk of developing breast cancer among women with BBD. To address this aim, data from a cohort of women with BBD from Washington County, Maryland enrolled in the CLUE-II study were analyzed.

Methods

CLUE II cohort

In 1989, a campaign named CLUE II ("Campaign against Cancer and Heart Disease") was conducted in Washington County, Maryland to establish a cohort with associated blood samples [30]. At baseline, participants signed a consent form, completed a brief medical and exposure history and a food frequency questionnaire, and donated a blood sample. The blood sample was collected in heparinzed tubes and centrifuged to obtain separation of the buffy coat which was then aliquotted and stored at -70°C. DNA was subsequently extracted from the buffy coat using standard phenol extraction [31].

A total of 25,081 persons (10,456 men and 14,625 women), about 30 percent of the Washington County residents, participated in the study. In addition to the information collected from this cohort at baseline in 1989, follow-up data were obtained from questionnaires administered in 1996 and approximately every 2 years thereafter. The Institutional Review Board at the Johns Hopkins Bloomberg School of Public Health approved this study.

BBD cohort

The BBD cohort is a sub-set of CLUE II. Details of the selection of CLUE II participants included in the BBD cohort are described elsewhere [32]. Briefly, women who responded on the 1996 CLUE II follow-up questionnaire that they had undergone a "breast biopsy or lumpectomy" were considered for inclusion into the BBD cohort. Women were included in the BBD cohort if either they were found to have BBD on their first located pathology report or a pathology report was not found but a breast biopsy was reported prior to or in the absence of a subsequent breast cancer diagnosis. Women who were diagnosed with breast cancer at their first biopsy, as reported by the participant or as determined using the pathology report search, were excluded from this analysis. In total, of the 1683 women who reported that they had a breast biopsy, 1467 women (87.2%) met the criteria above and were included in the BBD cohort. Among these 1467 women, pathology report data were collected for 362 (24.7%). Seventy percent of these pathology reports indicated a diagnosis of non-proliferative BBD, 26% indicated a diagnosis of proliferative disease without atypia, and 4% reported a diagnosis of proliferative disease with atypia.

For this analysis, 17 of the 1467 women were excluded because DNA could not be obtained from their stored blood samples and polymorphisms could not be genotyped. Further, all non-Caucasians (n = 12) were excluded from the analysis because previous studies have shown that race is an important confounder or effect modifier in investigations of polymorphisms and disease. These exclusions accounted from less than 1% of the BBD cohort. After applying these exclusions, the final analytic cohort included 1438 Caucasian women who were successfully genotyped for at least one of the genetic polymorphisms investigated in this study.

Outcome measurement

Incident cases of in situ or invasive breast cancer (International Classification of Diseases, Ninth Revision, code 233, 174) were identified through linkage of the cohort participants with the Washington County Cancer Registry and, since 1992, with the Maryland State Cancer Registry. The Washington County Cancer Registry identifies cancer cases from discharge records and pathology reports from Washington County Hospital, which is the only hospital in the county, and from death certificates. Since 1992, all hospitals cancer diagnostic laboratories, and radiation therapy centers in Maryland have been required to report incident cancer cases to the Maryland Cancer Registry, and currently, the Maryland Cancer Registry is certified as being more than 95% complete by the North American Association of Central Cancer Registries. While it is possible that cases of in situ or invasive breast cancer may have been missed due to migration out of the state after 1996, all women in the BBD cohort had at least 7 years of follow-up data (1989 to 1996). Further, approximately 80% of the BBD cohort responded to the 2000 follow-up questionnaire, indicating that the vast majority of the cohort remained under active surveillance in 2000.

Active case surveillance for the BBD cohort ended on April 28, 2003. In total, among all of the women included in the BBD cohort, 15 incident cases of in situ and 76 cases of invasive breast cancer were identified after the diagnosis of BBD.

Genotyping

Single nucleotide polymorphisms (SNPs) analyzed in the present study were selected as part of a larger study investigating the broad impact of genetic variation in candidate genes and their interactions with environmental exposures on cancer incidence and survival. For the larger study, polymorphisms that were suggested to alter function, encoded for a nonsynonymous amino acid change, or were located within the 5' or 3' untranslated region (UTR) of the gene and thus could potentially alter mRNA stability were chosen. Descriptions and dbSNP identifiers of the polymorphisms selected are shown on Table 1. Genotyping of the chosen SNPs in COMT, CYP1B1, CYP1A1, ESR1 and ESR2 was conducted at Applied Biosystems (ABI) and Celera Laboratories. All polymorphisms were genotyped using TaqMan technology (ABI, Foster City, CA, USA). The genotyping success rates of the polymorphisms selected ranged from 91.8% to 97.6%, with the exception of the CYP1B1 Arg48Gly polymorphism for which the genotyping success rate was 84.2%. The 84.2% genotyping success rate for CYP1B1 Arg48Gly polymorphism was due to a problem with the laboratory assay that was not resolved during the study period.

Table 1.

Description of single nucleotide polymorphisms examined in the progression of BBD to breast cancer

Gene dbSNP rs # snp description Amino Acid Substitution
COMT 4680 Ex3-12G>A Val158Met
CYP1A1 1048943 Ex7+131A>G Ile462Val
CYP1B1 1800440 Ex3+315A>G Asn453Ser
CYP1B1 10012 Ex2+143C>G Arg48Gly
CYP1B1 1056836 Ex3+251G>C Val432Leu
ESR1 1801132 Ex4-122G>C Pro325Pro
ESR1 2077647 Ex1+392T>C Ser10Ser
ESR1 746432 Ex1-192G>C Ala87Ala
ESR1 2273206 IVS6+52G>T
ESR1 851982 -104062C>T
ESR1 2228480 Ex8+229G>A Thr594Thr
ESR2 4986938 38 bp 3' of STP C>T
ESR2 928554 5659 bp 3' of STP G>A
ESR2 none 5696 bp 3' of STP A>G
ESR2 8018687 5772 bp 3' of STP A>G

Statistical analysis

The outcome variable examined in these analyses was the development of in situ or invasive breast cancer. Unconditional logistic regression was used to estimate age-adjusted odds ratios (ORs) and 95% confidence intervals (95% CIs) for the associations between the polymorphisms the development of breast cancer. Because previous studies indicate that the associations between several of the analyzed polymorphisms and the development of cancer may differ according to body mass index, smoking status, and alcohol intake, we conducted exploratory analyses to examine the associations between all of the polymorphisms and the development of breast cancer among strata of these variables (BMI: <25 kg/m2, ≥25 kg/m2; smoking status: ever, never; alcohol intake: current, no current use). Further, these analyses were conducted for all participants and for pre- and post-menopausal participants separately. Because the number of events among the pre-menopausal women was low (n = 24) and ORs for some of the genotypes could not be calculated, only the analyses for all participants and the post-menopausal subgroup are reported. As an additional exploratory analysis, logic regression [33] was employed using the software package R 2.0.1 to examine whether any interactions between the genotypes existed.

To address the issue of multiple testing in this study, p-values for the associations between single nucleotide polymorphisms and breast cancer risk were adjusted for the false discovery rate using the method proposed by Benjamini and Hochberg [34] in the software package R 2.0.1.

Unless otherwise specified, analyses were performed using SAS Version 8.2 (Cary, NC). A p-value of less than 0.05 was considered to be statistically significant.

Results

Characteristics of the analytic cohort are reported in Table 2. The mean age of the participants was 53.5 years (standard deviation 12.1), and the majority of the women had at least a high school degree (82.2%). Approximately 88% of the women had been pregnant at least once in their lifetime, 16.2% were current smokers, and 28.8% were current drinkers. Among the 1438 women in this sample, 91 (6.3%) developed invasive or in situ breast cancer after an initial breast biopsy for BBD.

Table 2.

Characteristics of the study cohort (n = 1438)

Characteristic n %
Race
 Caucasian 1438 100.0
Age, yearsa
 <50 533 37.1
 50 to 60 411 28.6
 >60 494 34.3
Missing 0 0.0
Education, yearsa
 less than a high school degree 259 18.0
 high school degree 714 49.7
 some college 463 32.2
Missing 2 0.1
Menopausal statusa
 Pre-menopausal 377 26.2
 Peri-menopausal 35 2.4
 Post-menopausal 995 69.2
Missing 31 2.2
Family history of breast cancera
 No 715 49.7
 Yes 275 19.1
Missing 448 31.2
Ever been pregnant (%)b
 No 176 12.2
 Yes 1255 87.3
Missing 7 0.5
Age at first birth (years, %)b
 Nulliparous 176 12.2
 20 347 24.1
 20 to 24 539 37.5
 ≥25 339 23.6
Missing 37 2.6
Age at menarche (years, %)b
 <12 268 18.6
 12 to 13 763 53.1
 >13 386 26.8
Missing 21 1.5
Height, inchesa
 <62 411 28.6
 62–64 419 29.1
 >64 608 42.3
Missing 0 0.0
Weight, poundsa
 <130 354 24.6
 130–<145 318 22.1
 145–<165 377 26.2
 ≥165 387 26.9
Missing 2 0.1
BMI, kg/m2, a
 <24.9 744 51.7
 25.0 – 29.9 433 30.1
 ≥30 259 18.0
Missing 2 0.1
Smoking statusa
 Never 839 58.3
 Former 366 25.5
 Current 232 16.1
Missing 1 0.1
Current alcohol drinkera
 No 814 56.6
 Yes 413 28.7
Missing 211 14.7

a data from 1989 questionnaire

b data from 1996 questionnaire

All of the polymorphisms examined were in Hardy-Weinberg equilibrium among women not developing breast cancer, with the exception of the CYP1B1 Ile462Val polymorphism (p-value = 0.02). Although statistically significant, the observed genotype counts for the CYP1B1 Ile462Val polymorphism were similar to the expected genotype counts under Hardy-Weinberg equilibrium (observed/expected: AA-1233/1229.5; AG-80/86.9; GG-5/1.5). All ESR2 polymorphisms were in strong linkage disequilibrium (D' > 90). Among the ESR1 polymorphisms, the Ser10Ser and Ala87Ala polymorphisms were strongly linked (D' > 90).

The associations between polymorphisms in the estrogen metabolizing enzymes and the risk of developing invasive breast cancer among women with BBD are shown in Table 3. Among all participants and post-menopausal participants only, carriers of at least one CYP1B1 453Ser allele had a borderline statistically significant increase in the risk of developing breast cancer compared to women carrying the referent Asn/Asn genotype (all participants: OR 1.48, 95% CI 0.95, 2.32; post-menopausal participants: OR 1.61; 95% CI 0.94, 2.74). The other polymorphisms in the estrogen metabolizing enzymes were not associated with breast cancer risk among women with BBD in this study. Results were not substantially altered by BMI, alcohol intake or smoking status (results not shown). No significant interactions between the genotypes were observed. To note, after adjustment for multiple testing, none of the associations between polymorphisms in the estrogen metabolizing enzymes and the risk of developing invasive breast cancer were statistically significant.

Table 3.

Associations between estrogen metabolizing polymorphisms and breast cancer risk in the BBD cohort

Cancer No Cancer
dbSNP rs# (n = 91) (n = 1347) All Participants Post-menopausal Only
n % n % Age- Adjusted OR (95% CI) Age- Adjusted OR (95% CI)

COMT Val158Met 4680
 GG 16 17.6 272 20.2 1.00 1.00
 GA 41 45.1 608 45.1 1.15 (0.63, 2.08) 0.89 (0.45, 1.77)
 AA 24 26.4 371 27.5 1.10 (0.57, 2.11) 0.90 (0.43, 1.90)
 GA/AA 65 71.4 979 72.7 1.13 (0.64, 1.98) 0.89 (0.47, 1.70)
 Missing 10 11.0 96 7.1
CYP1A1 Ile462Val 1048943
 AA 78 85.7 1233 91.5 1.00 1.00
 AG 7 7.7 80 5.9 1.38 (0.62, 3.10) 1.30 (0.45, 3.74)
 GG 1 1.1 5 0.4 3.33 (0.38, 28.99) 8.33 (0.74, 93.62)
  p-for-trend 0.20 0.20
 AG/GG 8 8.8 85 6.3 1.49 (0.70, 3.19) 1.56 (0.60, 4.08)
 Missing 5 5.5 29 2.2
CYP1B1 Asn453Ser 1800440
 AA 51 56.0 866 64.3 1.00 1.00
 AG 31 34.1 358 26.6 1.45 (0.91, 2.31) 1.51 (0.87, 2.65)
 GG 4 4.4 37 2.7 1.77 (0.61, 5.16) 2.44 (0.81, 7.36)
  p-for-trend 0.08 0.05
 AG/GG 35 38.5 395 29.3 1.48 (0.95, 2.32) 1.61 (0.94, 2.74)
 Missing 5 5.5 86 6.4
CYP1B1 Arg48Gly 10012
 CC 39 42.9 600 44.5 1.00 1.00
 CG 33 36.3 460 34.1 1.10 (0.68, 1.78) 0.95 (0.53, 1.69)
 GG 3 3.3 76 5.6 0.60 (0.18, 2.00) 0.25 (0.03, 1.88)
 CG/GG 36 39.6 536 39.8 1.02 (0.65, 1.64) 0.84 (0.48, 1.50)
 Missing 16 17.6 211 15.7
CYP1B1 Val432Leu 1056836
 CC 25 27.5 365 27.1 1.00 1.00
 CG 39 42.9 653 48.5 0.88 (0.53, 1.48) 1.04 (0.56, 1.98)
 GG 17 18.7 270 20.0 0.93 (0.49, 1.76) 0.93 (0.41, 2.09)
 CG/GG 56 61.5 923 68.5 0.90 (0.55, 1.46) 1.01 (0.56, 1.85)
 Missing 10 11.0 59 4.4

The associations between polymorphisms in ESR1 and ESR2 and the risk of developing invasive breast cancer among women with BBD are shown in Tables 4 and 5. A marginally significant decrease in the risk of developing breast cancer was observed among carriers of the ESR1 – 104062T allele compared to carriers of the referent genotype (all participants: OR 0.70, 95% CI 0.45, 1.09). Among all participants, the ESR2 *5772G allele was associated with a statistically significant decrease in the risk of breast cancer among women with BBD (OR 0.38; 95% CI 0.15, 0.96). A marginally significant increase in the risk of developing cancer was observed among women carrying at least one ESR2 *38A allele compared to the women homozygous for the GG genotype (all participants: OR 1.40; 95% CI 0.88, 2.25). OR estimates of the ESR2 *5772G and the ESR2 *38A polymorphisms were attenuated after adjustment for the presence of the other polymorphism (ESR2 *5772G OR 0.42; 95% CI 0.17, 1.05; ESR2 *38 OR 1.27; 95% CI 0.78, 2.04). Other ESR1 and ESR2 polymorphisms examined were not associated with breast cancer risk among women with BBD. Results did not differ substantially by BMI, alcohol intake or smoking status (results not shown). No significant interactions between the ESR1 and ESR2 genotypes were observed. After adjustment for multiple testing, the associations between the ESR1 and ESR2 polymorphisms and breast cancer described above were not statistically significant.

Table 4.

Associations between estrogen receptor-alpha (ESR1) polymorphisms and breast cancer risk in the BBD cohort

Cancer No Cancer
dbSNP rs# (n = 91) (n = 1347) All Participants Post-menopausal Only
n % n % Age- Adjusted OR (95% CI) Age-Adjusted OR (95% CI)

ESR1 Pro325Pro 1801132
 CC 52 57.1 794 58.9 1.00 1.00
 CG 31 34.1 440 32.7 1.07 (0.67, 1.69) 1.06 (0.61, 1.87)
 GG 7 7.7 64 4.8 1.65 (0.72, 3.78) 2.03 (0.81, 5.10)
 CG/GG 38 41.8 504 37.4 1.14 (0.74, 1.76) 1.19 (0.70, 2.01)
 Missing 1 1.1 49 3.6
ESR1 Ser10Ser 2077647
 TT 26 28.6 335 24.9 1.00 1.00
 TC 36 39.6 642 47.7 0.71 (0.42, 1.20) 0.90 (0.46, 1.77)
 CC 27 29.7 304 22.6 1.14 (0.65, 1.99) 1.88 (0.94, 3.75)
 TC/CC 63 69.2 946 68.8 0.85 (0.53, 1.37) 1.21 (0.65, 2.24)
 Missing 2 2.2 66 4.8
ESR1 Ala87Ala 746432
 GG 67 73.6 1077 80.0 1.00 1.00
 GC 15 16.5 181 13.4 1.32 (0.74, 2.36) 1.24 (0.61, 2.51)
 CC 1 1.1 7 0.5 2.30 (0.28, 18.95) 3.34 (0.38, 29.18)
  p-for-trend 0.3 0.3
 GC/CC 16 17.6 188 14.0 1.36 (0.77, 2.39) 1.31 (0.66, 2.60)
 Missing 8 8.8 82 6.1
ESR1 IVS6+52 2273206
 GG 69 75.8 1060 78.7 1.00 1.00
 GT 13 14.3 229 17.0 0.86 (0.48, 1.59) 0.71 (0.33, 1.53)
 TT 3 3.3 10 0.7 4.79 (1.29, 17.88) 5.31 (1.04, 27.28)
 GT/TT 16 17.6 239 17.7 1.02 (0.58, 1.79) 0.86 (0.43, 1.73)
 Missing 6 6.6 48 3.6
ESR1 Thr594Thr 2228480
 AA 2 2.2 41 3.0 1.00 1.00
 AG 20 22.0 358 26.6 1.14 (0.26, 5.05) 0.88 (0.19, 4.04)
 GG 58 63.7 841 62.4 1.42 (0.34, 6.01) 0.86 (0.20, 3.77)
 AG/GG 78 85.7 1199 89.0 1.34 (0.32, 5.62) 0.87 (0.20, 3.75)
 Missing 11 12.1 107 7.9
ESR1 – 104062C>T 851982
 CC 38 41.8 470 34.9 1.00 1.00
 CT 33 36.3 612 45.4 0.65 (0.40, 1.05) 0.55 (0.30, 0.99)
 TT 14 15.4 190 14.1 0.88 (0.47, 1.67) 0.89 (0.43, 1.85)
 CT/TT 47 51.6 802 59.5 0.70 (0.45, 1.09) 0.63 (0.37, 1.08)
 Missing 6 6.6 75 5.6

Table 5.

Associations between estrogen receptor-beta (ESR2) polymorphisms and breast cancer risk in the BBD cohort

Cancer No Cancer
(n = 91) (n = 1347) All Participants Post-menopausal Only
dbSNP rs# n % n % Age- Adjusted OR (95% CI) Age-Adjusted OR (95% CI)

ESR2 38 bp 3' of STP 4986938
 GG 26 28.6 470 34.9 1.00 1.00
 GA 43 47.3 612 45.4 1.27 (0.77, 2.10) 1.46 (0.80, 2.68)
 AA 19 20.9 190 14.1 1.83 (0.99, 3.38) 1.71 (0.78, 3.76)
  p-for-trend 0.06 0.1
 GA/AA 62 68.1 802 59.5 1.40 (0.88, 2.25) 1.52 (0.85, 2.71)
 Missing 3 3.3 75 5.6
ESR2 5659 bp 3' of STP 928554
 GG 10 11.0 202 15.0 1.00 1.00
 GA 44 48.4 632 46.9 1.41 (0.70, 2.86) 1.04 (0.48, 2.26)
 AA 28 30.8 419 31.1 1.38 (0.66, 2.89) 0.88 (0.38, 2.05)
 GA/AA 72 79.1 1051 78.0 1.40 (0.71, 2.76) 0.98 (0.47, 2.06)
 Missing 9 9.9 94 7.0
ESR2 5696 bp 3' of STP none
 AA 75 82.4 1101 81.7 1.00 1.00
 AG 12 13.2 180 13.4 0.96 (0.51, 1.81) 0.74 (0.33, 1.67)
 GG 1 1.1 4 0.3 3.68 (0.41, 33.37) --
 AG/GG 13 14.3 184 13.7 1.02 (0.56, 1.88) 0.73 (0.33, 1.64)
 Missing 3 3.3 62 4.6
ESR2 5772 bp 3' of STP 8018687
 AA 86 94.5 1133 84.1 1.00 1.00
 AG 5 5.5 169 12.5 0.39 (0.16, 0.99) 0.62 (0.24, 1.59)
 GG 0 0.0 5 0.4 -- --
 AG/GG 5 5.5 174 12.9 0.38 (0.15, 0.96) 0.61 (0.24, 1.55)
 Missing 0 0.0 40 3.0

Discussion

In this population-based cohort of women with BBD, there was evidence of an increased risk of breast cancer among women who carried the CYP1B1 453Ser allele compared to women who carried two copies of the CYP1B1 453Asn allele. None of the previously published studies on the CYP1B1 Asn453Ser polymorphism and breast cancer conducted among average-risk women reported an increase in risk of breast cancer associated with this polymorphism [35-38], including a recent meta-analysis that reported an OR of 0.91 (95% CI 0.79, 1.04) associated with the heterozygous Asn/Ser genotype and an OR of 0.85 (95% CI 0.54, 1.34) associated with the homozygous Ser/Ser genotype [39]. However, functionality studies demonstrate that the CYP1B1 polymorphic variant is associated with both higher catalytic activity in converting estrogen to 4-hydroxy estrogens and greater levels of DNA damage [39-41]. This mechanism may be more relevant for progression among the subgroup of women with BBD who progress to breast cancer, thus it is reasonable to examine this association among women biopsy proven BBD.

A marginally significant positive association was observed for the ESR2 *38G>A. This finding is not consistent with results of published studies among either average-risk or high-risk women. Maguire et al [26] reported no increase in breast cancer risk associated with two copies of the variant *38A allele among average-risk (OR 0.81; 95% CI 0.50, 1.31) or high risk (OR 1.00; 95% CI 0.58, 1.71). In addition, Gold et al [16] observed that haplotypes containing the common ESR2 *38G allele were associated with an increased risk of breast cancer among Ashkenazi Jews. These differences in findings may be due to the different populations under study; Maguire et al [26] examined ESR2 polymorphisms among patients in Sweden and Gold et al (16) investigated ESR2 and breast cancer among the Ashkenazi Jews. Neither investigated the association of ESR2 polymorphisms among women diagnosed with BBD.

In addition, results from this study suggest that women with BBD who carry the ESR2 *5772A>G polymorphism or the ESR1 – 104062C>T polymorphism are at decreased risk of developing breast cancer. To our knowledge, neither of these genotypes has been examined in women with BBD or among average risk women. The regions surrounding each polymorphism are well conserved with little recombination, therefore, it likely that, if the associations are real, the observed associations are due to linkage disequilibrium with another functional polymorphism in the region. No information on functionality is know for either ESR2 *5772A>G or ESR1 – 104062C>T.

There was no evidence of an association between the other polymorphisms examined in this study, including those in COMT and CYP1A1, and breast cancer risk. Although no published study has investigated the COMT Val158Met and CYP1A1 Ile462Val polymorphisms in the progression of BBD to invasive breast cancer, previous studies of average-risk women have reported discrepant results regarding the association between the COMT Val158Met and the CYP1A1 Ile462Val polymorphisms and the risk of breast cancer [8,42]. Both polymorphisms have been observed to be functional; the COMT 158Met allele is associated with three- to four-fold decreased activity compared to the wildtype allele [43] and the CYP1A1 462Val allele is consistent with higher enzyme activity [44]. Therefore, an association between these polymorphisms and breast cancer is biologically plausible and support the findings of studies that show an association between the polymorphisms and breast cancer risk. It may be, however, that both polymorphisms only modify the association between endogenous estrogens and the risk of breast cancer. Incorporating data on circulating estrogen concentrations may clarify the importance of carrying a specific genotype. Alternatively, it may also be that the effect of any single polymorphisms on the risk of breast cancer is small and that it is necessary to look at combinations of variants in the hormone metabolism pathway.

While this study provides novel information regarding the role of polymorphisms in estrogen metabolizing enzymes and the estrogen receptor genes in the progression of BBD to breast cancer, this study has several limitations inherent to its design. As reported in a previously published investigation on this cohort of women [32], pathology reports were not able to be obtained for all women who reported that they had undergone a surgical biopsy. This was due both to difficulties in obtaining permission for pathology review for some participants as well as to an inability to obtain records of biopsies done more than 15 to 20 years ago. Since concordance of finding a pathology report and report of biopsy among women granting permission for pathology review who reported that they had undergone a biopsy after 1980 was high (92.5%), all women who reported a breast biopsy were included in the analyses. However, this may have led to the inclusion of a small number of women without BBD. Further, because data on the type of BBD were not collected for all participants, the analyses conducted in this study were not stratified by type of BBD, and, therefore, the ORs reported may underestimate (or overestimate) the true associations among women with certain types of BBD.

In addition, though the base cohort is relatively large, the number of cases of breast cancer occurring limited the power of the study to make firm conclusions about the relationships between polymorphisms in COMT, CYP1B1, CYP1A1, ESR1 and ESR2 and the risk of breast cancer in Caucasian women with BBD. We had limited power to detect small associations and, therefore, were also limited in our ability to correct for multiple testing. As stated in the results section, the associations between the polymorphisms and the risk of developing breast cancer were not statistically significant after correction for multiple testing and this may have been due, in part, to the small sample size. However, while we may be able to rule out large changes in risk of clinical and public health consequence associated with certain genotypes, we still observed, with the small number of events, statistically significant changes in the risk of breast cancer in this cohort. Taken together with functional considerations of these polymorphisms, it is important to follow-up on these observations to determine if we can better understand and perhaps intervene for those women with BBD who are most at risk to progress to cancer.

Conclusion

The findings of this study indicate that specific polymorphisms in the CYP1B1, ESR1, and ESR2 genes may play a role in progression of BBD to breast cancer among Caucasian women. Although additional studies are needed to confirm or refute our findings, these results suggest that genetic markers may aid in the identification of women who are at risk for progression of BBD to cancer.

Abbreviations

BBD Benign breast disease

COMT Catechol O-methyltransferase

CYPs Cytochrome P450 enzymes

ESR1 Estrogen receptor-alpha

ESR2 Estrogen receptor-beta

SNP Single nucleotide polymorphism

Competing interests

The author(s) declare that they have no competing interests.

Authors' contributions

LG contributed to the statistical analysis, interpretation of the data, and the writing of the manuscript. SIB provided expertise on the more advanced analyses of the genetic data and contributed to the interpretation of the data. MAM, LWT, and SAH contributed to the data collection and statistical analysis. PA conducted reviews of the pathology report data and pathology specimens. CJN and KJN contributed to the conception and design of the study and the interpretation of the data.

Pre-publication history

The pre-publication history for this paper can be accessed here:

http://www.biomedcentral.com/1471-2407/6/173/prepub

Acknowledgments

Acknowledgements

This research was supported by a National Cancer Institute SPORE grant CA8843 and a National Institute on Aging grant AG18033 from the National Institutes of Health. The funding agencies had no role in the study design, collection, analysis and interpretation of the data, or in the writing of the manuscript. Dr. Gallicchio is supported by an Institutional National Research Service Award from the National Cancer Institute (T32 CA09314). The authors thank Dr. Ingo Ruzcinski for providing his biostatistics expertise in this analysis. The authors thank Judy Bolton-Hoffman and Alyce Burke at the Comstock Center for Public Health Research and Prevention for their help in carrying out this study.

Contributor Information

Lisa Gallicchio, Email: lgallic@mdmercy.com.

Sonja I Berndt, Email: sberndt@jhsph.edu.

Meghan A McSorley, Email: mcsorley.meghan@medstudent.pitt.edu.

Craig J Newschaffer, Email: cnewscha@jhsph.edu.

Lucy W Thuita, Email: lthuita@jhsph.edu.

Pedram Argani, Email: pargani1@jhmi.edu.

Sandra C Hoffman, Email: shoffman@jhsph.edu.

Kathy J Helzlsouer, Email: khelzlso@mdmercy.com.

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