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Dietary and Plasma Lycopene and the Risk of Breast Cancer

Divisions of ¹ Preventive Medicine and ² Aging, Department of Medicine, Brigham and Women's Hospital and Harvard Medical School; ³ Massachusetts Veterans Epidemiology Research and Information Center, VA Boston Healthcare System; ⁴ Department of Epidemiology, Harvard School of Public Health, Boston, Massachusetts; and ⁵ Departments of Medical Research, Our Lady of Mercy Medical Center and Community and Preventive Medicine, New York Medical College, Bronx, New York

Requests for reprints: Howard D. Sesso, Division of Preventive Medicine, Brigham and Women's Hospital, 900 Commonwealth Avenue East, Boston, MA 02215-1204. Phone: 617-732-8837; Fax: 617-734-1437. E-mail: hsesso{at}hsph.harvard.edu

	Abstract

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Lycopene is potentially effective in the prevention of breast cancer from laboratory and observational studies. Among 39,876 women initially free of cardiovascular disease and cancer, we first conducted a prospective cohort study of dietary lycopene and its food sources. Participants completed a baseline food frequency questionnaire and provided self-reports of breast cancer risk factors. Dietary lycopene levels were divided into quintiles, and lycopene food sources were categorized. During 9.9 years of follow-up, 1,076 breast cancer cases were confirmed by medical record review. In a nested case-control study, we then identified 508 breast cancer cases and 508 controls matched by age, smoking, and follow-up time. Plasma lycopene and other carotenoids were measured. In the prospective cohort study, women with increasing quintiles of dietary lycopene had multivariate relative risks (RR) of breast cancer of 1.00 (ref), 0.95, 1.00, 1.10, and 1.00 (P, linear trend = 0.71). Women consuming <1.5, 1.5 to <4, 4 to <7, 7 to <10, and 10 servings/week of tomato-based products had RRs of 1.00 (ref), 1.00, 1.20, 1.18, and 1.16 (P, linear trend = 0.11). No individual lycopene food sources were associated with breast cancer. In the nested case-control study, women in increasing quartiles of plasma lycopene had multivariate RRs of breast cancer of 1.00 (ref), 0.95, 1.15, and 0.93 (P, linear trend = 0.86). The stepwise addition of individual plasma carotenoids did not impact the RRs for plasma lycopene, nor were other carotenoids associated with breast cancer. In conclusion, neither higher dietary nor plasma lycopene levels were associated with a reduced risk of breast cancer in middle-aged and older women.

	Introduction

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There is considerable epidemiologic evidence supporting an association between higher levels of fruit and vegetable intake and a reduced risk of total cancer (1). With regard to breast cancer, the evidence is not consistent based on two metaanalyses (2, 3). Specific nutrients rich in fruits and vegetables, including carotenoids, may play a role in breast cancer prevention. Recently, lycopene has garnered specific attention over other carotenoids for its potential role in cancer prevention. Lycopene is a carotenoid without provitamin A activity and is found in a limited number of plant foods (tomato, watermelon, pink grapefruit, papaya, apricot). More than 80% of lycopene intake in the U.S. is obtained from the consumption of tomatoes and tomato products (4), making it more amenable to potential public health strategies to increase intake.

Various studies have also explored promising mechanisms through which lycopene, independent of other carotenoids, may have a role in reducing the risk of breast cancer. Lycopene has been shown to have strong antioxidant properties relative to other carotenoids (5). Lycopene may inhibit the proliferation of mammary human cancer cells (6). Alternatively, lycopene may suppress insulin-like growth factor-I (7), which has been linked to increased risk of premenopausal breast cancer (8). No study has examined lycopene's role for breast cancers positive for steroid hormone receptors (6). Observational evidence from several case-control and cohort studies that examined the association between dietary, blood, or adipose tissue levels of lycopene and the risk of breast cancer has remained inconsistent, along with the findings for other carotenoids (9-21). However, there are no published data specifically examining the association between the consumption of lycopene-containing foods and the risk of breast cancer.

With the availability of both dietary and plasma assessments of lycopene from the Women's Health Study, we simultaneously focused on the roles of dietary consumption of lycopene-containing foods and plasma lycopene in breast cancer risk using corresponding prospective cohort and nested case-control study designs.

	Materials and Methods

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Study Population
The Women's Health Study is a 2 x 2 factorial trial of low-dose aspirin and vitamin E in the primary prevention of cardiovascular disease and cancer (22). The ß-carotene component of the trial was terminated in 1996 due in part to the lack of an effect of ß-carotene on cancer incidence in the Physicians' Health Study (23, 24). A total of 39,876 female U.S. health professionals, aged 45 years in 1992 and free from prior myocardial infarction, stroke, transient ischemic attack, and cancer (except nonmelanoma skin cancer) were enrolled and randomized into the study. The Institutional Review Board at Brigham and Women's Hospital approved the study protocol and informed consent was obtained for each subject.

Prospective Cohort Study of Dietary Lycopene and its Food Sources
Among those randomized into the Women's Health Study, a 131-item validated Willett semiquantitative food frequency questionnaire was completed by 39,310 women (25), of whom 829 were excluded due to insufficient completion of the questionnaire, or because their daily energy intake was <2,510 or 14,644 kJ/day (<600 or 3,500 kcal/day). After an additional exclusion of those with a pre-randomization revascularization procedure, 38,447 women remained for analyses of dietary lycopene.

Baseline Covariates
On the Women's Health Study baseline questionnaire, women provided self-reported data on age, weight, and height (converted to body mass index, in kg/m²), smoking status, alcohol intake, frequency of exercise, family history of breast cancer in first-degree relatives, age at menarche, history of oral contraceptive use, age at first pregnancy, number of pregnancies, postmenopausal status, and postmenopausal hormone use.

On the semiquantitative food frequency questionnaire, a common unit or portion size for each food was specified, and the participants selected from nine responses ranging from "never or less than once per month" to "6 + per day." Dietary lycopene intake, adjusted for total energy intake using the residual method (25), was calculated in micrograms per day and based on food tables maintained by the Harvard School of Public Health, Boston, MA. Other studies have reported moderate-to-high correlations between the semiquantitative food frequency questionnaire and dietary records for lycopene food sources (26, 27). Four major lycopene food sources were also considered, including tomatoes, tomato juice, tomato sauce, and pizza. Other nutrients and foods considered for analyses included total fiber, folate, and saturated fat intake, which were also adjusted for total energy intake, plus total fruit and vegetable intake.

Ascertainment of Breast Cancer
Women completed follow-up questionnaires every 6 months during the first year, then annually thereafter during the course of the study. Women reported a diagnosis of breast cancer either through these follow-up questionnaires, by letter, or by telephone. Family members or postal authorities usually reported deaths. Medical records were obtained for all reported cases of breast cancer, with an Endpoints Committee of physicians to confirm or refute the occurrence of breast cancer. Additional details on breast cancer (e.g., hormone receptor status) were also abstracted. Only confirmed cases of invasive and in situ breast cancer were included.

Nested Case-Control Study of Plasma Lycopene
Baseline blood samples were collected from 28,345 (71%) participants and stored in liquid nitrogen freezers until analysis. A nested case-control study was conducted, identifying 508 case-control pairs with baseline blood samples. Cases included women developing breast cancer confirmed by an Endpoints Committee during a mean of 7 years of follow-up. Each case was then matched with a control subject according to age (± 1 year), smoking status (never, former, and current smoker), and follow-up time (± 6 months), while remaining free of breast cancer throughout follow-up.

All investigators and laboratory personnel were blinded to the subject's case-control status, and blood samples were handled identically. Baseline plasma blood samples were thawed and assayed for lycopene and other carotenoids at Our Lady of Mercy Medical Center, Bronx, NY. All analytes were quantitated by reversed-phase high-performance liquid chromatography following extraction and concentration by conventional methodology (28). Plasma total cholesterol was assayed by enzymatic, end point spectroscopy using commercially available diagnostic kits (Sigma-Aldrich Chemical, Co., St. Louis, MO) and conventional methodology (29, 30). Because plasma lipoproteins are nonspecific carriers for all plasma carotenoids, the measurement of total cholesterol represents the best way to control for the confounding effects due to differences in lipoprotein levels between subjects (31). Although confounding by total cholesterol is largely unknown for breast cancer, we took a conservative data analysis approach and controlled for plasma cholesterol.

Laboratory performance was based on blind quality control samples provided from both the Women's Health Study and the Department of Pathology Quality Assurance program at Our Lady of Mercy Medical Center, and on repeated assays of laboratory-prepared sample pools. Several blind quality control samples and laboratory pools were assayed with each analysis run to monitor laboratory performance. The laboratory accuracy was within 7% for each measured carotenoid, whereas the day-to-day and within-day precision (coefficient of variation) for these analytes was 5% (32).

Data Analyses
For the prospective cohort study, lycopene intake was grouped by quintiles based on its overall distribution of intake. Participants were first compared by quintile of lycopene intake, using mean values or proportions of baseline coronary risk factors. Cox proportional hazards modeled the relative risk (RR) and 95% confidence interval (CI) of breast cancer, with the lowest quintile as the reference. The 95th percentile versus lowest quintile of lycopene intake was also compared. Models were first adjusted for age, total energy intake, and randomized treatment assignments, then life-style and clinical factors, and finally by dietary factors. Linear trends across quintiles of lycopene intake were tested using the median level for each quintile as an ordinal variable.

Categories of major lycopene food sources paralleled a previous study from the Women's Health Study (33): tomatoes (one serving = one tomato), none, 1 to 3 servings/month, 1 to 4 servings/week, 5 servings/week; tomato juice (small glass), none, 1 to 3 servings/month, 1 serving/week, and 2 servings/week; tomato sauce (1/2 cup or 118 mL), none, 1 to 3 servings/month, 1 serving/week, and 2 servings/week; and pizza (2 slices), none, 1 to 3 servings/month, 1 serving/week, and 2 servings/week. Serving sizes reflect what is mentioned on the semiquantitative food frequency questionnaire, and the categories were determined a priori based on the distribution of intake for each lycopene food source. We summed the total number of tomato-based products as <1.5, 1.5 to <4, 4 to <7, 7 to <10, and 10 servings/week (34). These analyses included total energy intake in each model. The proportional hazards assumption was satisfied using a Wald test for the interaction of time with each lycopene indicator variable.

For the nested case-control study, women were first compared according to case-control status. Plasma lycopene levels were then divided into quartiles based on its distribution among 508 controls, for which baseline characteristics were compared. We computed the RRs and 95% CIs of breast cancer using conditional logistic regression for increasing quartiles of plasma lycopene levels, with the lowest quartile as the reference. Linear trends across quartiles of plasma lycopene levels were tested using the median level for each quartile as an ordinal variable. Models were first adjusted for randomized treatment assignments and plasma total cholesterol level, then adjusted sequentially for life-style, clinical, and dietary factors as done for the cohort study. We also considered whether simultaneous adjustment for other plasma carotenoids attenuated the association between plasma lycopene and breast cancer. Other analyses were limited to cases that were positive for estrogen and progesterone receptors (344 case-control pairs). Finally, multivariate models were then compared for plasma lycopene with other carotenoids categorized into quartiles among the controls and entered into a separate model.

	Results

Top Abstract Introduction Materials and Methods Results Discussion References

 
Prospective Cohort Study of Dietary Lycopene and its Food Sources
Overall, the mean (SD) lycopene intake was 9,199 (6,443) µg/day in 38,447 women aged 53.9 (7.0) years. Both tomato sauce (40.5%) and tomatoes (39.8%) were the major food sources of dietary lycopene intake, followed by tomato juice (12.3%), pizza (4.7%), grapefruit (2.7%), and salsa (0.1%). Table 1 compares selected baseline characteristics of women according to their quintiles of lycopene intake. Higher dietary lycopene intake was associated with slightly lower body mass index, smoking rates, and family history of breast cancer, and was only weakly associated with reproductive risk factors. Women consuming greater amounts of lycopene also exercised more and consumed greater amounts of fruits and vegetables, fiber, and folate, as well as less saturated fat.

We next examined the association between increasing quartiles of plasma lycopene and the risk of breast cancer (Table 5). Crude models matched for age and smoking status, as well as multivariate models each showed no association between plasma lycopene and the risk of breast cancer (all P, linear trend >0.05). Controlling for potential confounders of the association between plasma lycopene and breast cancer only attenuated the RRs in the highest quartile. We also examined plasma lycopene and the risk of breast cancers that were positive for estrogen and progesterone receptors in 344 case-control pairs of women. In fully adjusted models, there was still no association between higher levels of plasma lycopene and a lower risk of breast cancer with a positive receptor status (P trend = 0.80).

Quartiles of plasma carotenoids aside from plasma lycopene were also considered for their independent multivariate associations with the risk of breast cancer in Table 6. As with models for plasma lycopene, there was very little confounding of the association between each plasma carotenoid and risk of breast cancer. Higher quartiles of neither - nor ß-carotene were associated with the risk of breast cancer in multivariate models (both P trend >0.05). Women with elevated levels of plasma ß-cryptoxanthin and lutein/zeaxanthin had slight nonsignificant reductions in the risk of breast cancer compared with those in the lowest quartile.

	Discussion

Top Abstract Introduction Materials and Methods Results Discussion References

Epidemiologic studies assessing whether dietary (9-13) or blood (14-17) lycopene are associated with the risk of breast cancer have provided no clear answer. Numerous other studies have examined not only lycopene but also other dietary and blood carotenoids, with equally inconsistent results (37). Among studies of dietary lycopene, only a Swiss case-control study (289 cases) reported a strong inverse association with breast cancer (38). On the other hand, previous long-term prospective studies of dietary lycopene consumption among Canadian (10) and U.S. (11, 13, 39) women have found no association with pre- and postmenopausal breast cancer risk. The present study is the first to additionally examine the role of tomato-based food products with the risk of breast cancer, and no association was apparent.

Among studies of serum and plasma lycopene, a nested case-control study of U.S. women (295 cases) found a strong association between plasma lycopene and breast cancer risk (15). In another nested case-control study of Swedish women (201 cases) selected from multiple cohorts, an inverse association (P trend = 0.01) between plasma lycopene and breast cancer was limited to a subcohort of only 67 postmenopausal cases (16). In contrast, two case-control studies of serum lycopene found no association with breast cancer (14, 17).

The finding of only a modest correlation between dietary intake of lycopene and plasma lycopene levels (Spearman r = 0.25) suggests that our attempt to directly associate diets that are simply rich in lycopene with higher plasma lycopene levels may be too simplistic. In support of this suggestion, we also reported a weak but significant correlation of 0.14 in another nested case-control study using data from the Women's Health Study (32). Lycopene in foods occurs mainly in the thermodynamically stable all-trans form (40), whereas the more unstable cis-isomer accounts for 50% to 70% of total lycopene in human plasma (40, 41). To further confound the issue, others have reported the correlation between dietary lycopene intake and plasma lycopene to be stronger in men than in women (42, 43). For example, among 162 nonsmoking women in the Nurses' Health Study, the adjusted correlation was 0.21 for lycopene, whereas in 110 nonsmoking men from the Health Professionals Follow-up Study the correlation was 0.47 (42). Reasons for this gender disparity remain unclear. One possible explanation for the lower correlations between dietary lycopene intake and plasma lycopene in studies may include differences in actual dietary patterns, which include lower intakes of tomato sauce that contain lycopene in a more bioavailable food matrix (34, 44).

Despite our lack of association for lycopene and breast cancer, lycopene may still have chemopreventive properties. Research suggests that lycopene strongly inhibits the proliferation and cell cycle proliferation of mammary human cancer cells (6) and suppresses insulin-like growth factor-I (7), which has been strongly linked with an increased risk of breast cancer in premenopausal women in some studies.

We considered the association between dietary lycopene intake and plasma lycopene with the risk of breast cancers that were positive for steroid hormone receptors based on previous findings to suggest that estrogen receptor status is an important factor for breast cancer cell response to carotenoids, including lycopene (6). We hypothesized that if lycopene or other carotenoids had a role in the prevention of breast cancer through an endogenous hormonal mechanism, a stronger inverse association would be observed for women positive for estrogen and progesterone receptors. However, based on our findings for both dietary lycopene intake and plasma lycopene, we found no evidence to support this mechanism.

A number of potential limitations of the present study also warrant discussion. First, we relied on a single baseline measurement of dietary or plasma lycopene, raising the possibility of regression to the mean that could bias our RRs toward the null hypothesis and underestimate the observed risk reductions. However, total plasma lycopene has been shown to be reasonably stable in samples taken 3 to 4 years apart with a correlation of 0.63 (45). Furthermore, even with the use of repeated dietary lycopene measurements, no association remained with breast cancer among U.S. nurses (11). Second, we have not directly assessed the long-term stability of plasma lycopene stored at –140°C in liquid nitrogen–chilled freezers since 1993. However, studies comparing measurements of plasma lycopene and other carotenoids support the long-term stability of these biochemical markers (46, 47). Third, the women in our study did not consume large amounts of specific tomato-based food products, resulting in narrow distributions of intake and lower levels of plasma lycopene. This fact may have limited our ability to discern possible dose-response or threshold effects that might have been present in our data. Finally, residual confounding may also be of concern, but seems unlikely. We comprehensively controlled or matched for major breast cancer risk factors, which had a trivial impact on the reported RRs.

In summary, neither higher dietary nor plasma lycopene levels were associated with a reduced risk of breast cancer in this population of middle-aged and older female health professionals. Despite promising mechanistic studies, this large-scale study of dietary lycopene, tomato-based food products, and plasma lycopene does not support a role for lycopene in breast cancer carcinogenesis.

	Acknowledgments

 
The authors would like to acknowledge the crucial contributions of the entire staff of the Women's Health Study, under the leadership of David Gordon, and of the Women's Health Study Endpoints Committee (Drs. I-Min Lee and Wendy Y. Chen). We are also indebted to the 39,876 dedicated and committed participants of the Women's Health Study.

	Footnotes

 
Grant support: Research grants CA-47988 and HL-43851 from NIH, Bethesda, MD, and from Roche Vitamins, Inc.

The costs of publication of this article were defrayed in part by the payment of page charges. This article must therefore be hereby marked advertisement in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.

Received 9/20/04; revised 1/27/05; accepted 2/11/05.

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