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Genetic Variants of DNA Repair Genes and Prostate Cancer: A Population-Based Study

¹ George Washington University School of Public Health and Health Services, Washington, District of Columbia; ² Division of Cancer Epidemiology and Genetics, National Cancer Institute, NIH, Bethesda, Maryland; ³ Celera Diagnostics LLC, Alameda, California; ⁴ Shanghai Cancer Institute, Shanghai, China; and ⁵ Department of Obstetrics and Gynecology, Keck School of Medicine, University of Southern California, Los Angeles, California

Requests for reprints: Ann W. Hsing, Division of Cancer Epidemiology and Genetics, National Cancer Institute, NIH, EPS-MSC 7234, 6120 Executive Boulevard, Bethesda, MD 20892-7234. Phone: 301-496-1691; Fax: 301-402-0916. E-mail: hsinga{at}mail.nih.gov

	Abstract

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As part of a population-based case-control study in Shanghai, China, we investigated whether variants in several DNA repair genes, either alone or in conjunction with other risk factors, are associated with prostate cancer risk. Genomic DNA from 162 patients newly diagnosed with prostate cancer and 251 healthy men randomly selected from the population were typed for five nonsynonymous DNA repair markers. We found that the XRCC1-Arg399Gln AA and the MGMT-Leu84Phe CT+TT genotypes were associated with an increased risk of prostate cancer [odds ratio (OR), 2.18; 95% confidence interval (CI), 0.99-4.81 and OR, 1.99; 95% CI, 1.19-3.34, respectively]. In contrast, XRCC3-Thr241Met, XPD-Lys751Gln, and MGMT-Ile143Val markers showed no significant associations with risk, although due to the much lower frequency of their variant alleles in this population we cannot rule out small to modest effects. There was a significant interaction between the MGMT-84 marker and insulin resistance (P_interaction = 0.046). Relative to men with the MGMT-84 CC genotype and a low insulin resistance (<0.097), those having the CT-TT genotype and a greater insulin resistance had a 5.4-fold risk (OR, 5.39; 95% CI, 2.46-11.82). In addition, for the XRCC3-241 marker, relative to men with the CC genotype and a low intake of preserved foods (<12.7 g/d), those harboring the CT+TT genotype and having a higher intake of preserved foods (>12.7 g/d), which contain nitrosamines and nitrosamine precursors, had a significantly increased risk of prostate cancer risk (OR, 2.62; 95% CI, 1.13-6.06). In contrast, men with the CT+TT genotype and a low intake of preserved foods had a 69% reduction in risk (OR, 0.31; 95% CI, 0.10-0.96; P_interaction = 0.005). These results suggest that genetic variants in the DNA repair pathways may be involved in prostate cancer etiology and that other risk factors, including preserved foods and insulin resistance, may modulate prostate cancer risk in combination with genetic susceptibility in these repair pathways. Replication in larger studies is necessary to preclude chance findings, particularly those among subgroups, and clarify the mechanisms involved.

	Introduction

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Prostate cancer is the most common cancer diagnosed among men in the United States. In 2005, an estimated 232,090 new cases will be diagnosed and 30,350 men will die from prostate cancer in the United States (1). African-Americans have the highest reported rates of prostate cancer in the world, with an age-adjusted rate of 137 per 100,000, which is 60 times higher than the reported incidence in Shanghai, China, where the reported incidence is the lowest in the world at 2 per 100,000 (2, 3). Reasons for the large racial differences in prostate cancer risk are unclear.

Although several factors have been implicated in prostate cancer etiology, only age, race, and a family history of prostate cancer are established risk factors. Data from previous twin and family studies suggest a genetic component for prostate cancer (4). To date, six rare, highly penetrant loci have been identified; however, these loci are estimated to be responsible for only 5% to 10% of all prostate cancer cases (5, 6). More common polymorphisms, such as those in DNA repair genes, may account for a larger proportion of prostate cancer in the population despite having a lower penetrance and conferring a much lower prostate cancer risk on individuals (7, 8).

Genomic stability and integrity are important in maintaining accurate DNA replication. DNA disruptions can lead to gene rearrangements, translocations, amplifications, and deletions, which can in turn contribute to cancer development (9, 10). DNA is assaulted on a daily basis by a variety of endogenous processes and exogenous factors, including UV light, cigarette smoke, dietary factors, reactive oxygen species, and carcinogens, all of which can cause varying degrees of DNA damage and lead to DNA mutation (11). DNA repair mechanisms defend against these exogenous insults, correcting DNA damage as well as normal replication errors.

There are a number of DNA repair pathways, each responsible for repairing a different type of DNA damage. Base excision repair removes simple base modifications, including single-strand breaks, oxidative DNA damage, and alkylation and nonbulky adducts (12). Nucleotide excision repair removes larger lesions, which often result from environmental damage, including UV radiation and external carcinogens (13). Alkyltransferases directly reverse DNA damage by transferring alkyl groups from damaged DNA onto the transferase enzyme (14). Double-stranded DNA breaks are repaired through mechanisms including the homologous recombination repair pathway (15).

To clarify further the role of DNA repair pathways in prostate carcinogenesis, we investigated common nonsynonymous single nucleotide polymorphisms (SNP) in four DNA repair genes in a population-based case-control study in Shanghai, China. These genes, all previously studied in relation to other malignancies, include the X-ray repair cross-complementary group 1 (XRCC1)-Arg399Gln (G to A), involved in base excision repair; the XRCC3-Thr241Met (C to T), involved in homologous recombination repair; the O⁶-methylguanine-DNA-methyltransferase (MGMT)-Ile143Val (A to G) and MGMT-Leu84Phe (C to T), involved in direct damage reversal; and the xeroderma pigmentosum group D (XPD)-Lys751Gln (A to C), involved in nucleotide excision repair (16-18).

We also examined the combined effects of these DNA repair variants with a number of risk factors that have been reported in this study population. For example, in earlier reports, we have shown that abdominal obesity (measured by waist-to-hip ratio), insulin resistance (measured by the ratio of fasting serum insulin to glucose levels), and consumption of preserved foods are associated with a significant excess risk of prostate cancer in Chinese men and that consumption of allium vegetables is associated with a lower risk (19-21). Obesity and insulin resistance are closely linked to chronic inflammation, which may result in DNA damage (22, 23). Salted and preserved foods contain nitrosamines and nitrosamine precursors that induce DNA damage that is mitigated by DNA repair mechanisms (22, 23). Also, organosulfur compounds in allium vegetables may directly modulate DNA repair capacity (24). Thus, in this report, we evaluated the individual and combined effect of DNA repair allelic variants with these risk factors on prostate cancer risk.

	Materials and Methods

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Study Population
Details of this population-based case-control study have been reported previously (19, 20). Briefly, cases were permanent residents of Shanghai newly diagnosed with prostate cancer (ICD-9 185) between 1993 and 1995, identified through a rapid reporting system in 28 collaborating hospitals in urban Shanghai. Cases had no previous history of cancer. Four cases were excluded from the study after Chinese and American pathologists jointly confirmed them to be benign prostatic hyperplasia. The rapid reporting system captured over 95% of the cases diagnosed in urban Shanghai during the study period. Based on records maintained at the Shanghai Resident Registry, male controls with no history of cancer were selected at random from the 6.5 million permanent Shanghai residents over 18 years of age and frequency matched to cases by age (5-year intervals). This study was approved by the Institutional Review Boards at the National Cancer Institute, the Shanghai Cancer Institute, and the George Washington University School of Public Health and Health Services.

Interview
Using a structured questionnaire, trained personnel conducted in-person interviews to collect information on demographic characteristics, diet and smoking history, consumption of alcohol and other beverages, medical history, family cancer history, physical activity, and sexual behavior. Diet was assessed by means of a 122-item food frequency questionnaire developed for and validated in the Shanghai population. Based on the 122 food items, over 40 food groups, including preserved food, meat, and vegetable groups, were derived (20). The Chinese Food Composition Table was used to derive nutrient indices for each food item and computation of total calories. As another part of the interview, anthropometric measurements were taken, including waist and hip circumferences and height and weight (19). A total of 243 of 264 eligible cases and 472 of 495 eligible controls were interviewed.

Blood Collection and DNA Extraction/Laboratory Analysis
Two-hundred interviewed cases and 330 interviewed controls provided overnight fasting (before 10 a.m.) blood samples for the study. Blood samples were processed and separated within 2 hours of collection at a central laboratory in Shanghai. The blood fractions were stored at –70°C in Shanghai before shipment to the United States on dry ice. DNA was extracted from the buffy coat fractions at the American Type Culture Collection (Manassas, VA). The samples were genotyped at the National Cancer Institute laboratory. Levels of fasting insulin and glucose were measured at F. Stanczyk's laboratory, using commercially available RIA kits (Linco Research, St. Charles, MO). The coefficients of variation of these assays were <8%. The ratio of insulin to glucose was used as an index of insulin resistance (21). For both the genotyping and biomarker assays, laboratory personnel were masked to case-control status in the arrangement of biospecimens.

Molecular Analysis and Assessment of DNA Repair Genes
The selected SNPs were analyzed in 162 cases and 251 controls who had sufficient DNA available using a combination of matrix-assisted laser desorption ionization time of flight (MALDI-TOF) mass spectrometry and Homogeneous MassExtend chemistry (Sequenom, San Diego, CA). SpectroDesigner Software (Sequenom) was used for assay design. Two MALDI-TOF/Homogeneous MassExtend multiplex assays that included the five studied SNPs were selected according to optimum assay partners, reaction terminator mixes, and primers both for genomic PCR amplification of the SNP-containing sequences and DNA polymerase extension within the optimal mass range of 5,000 to 8,500 Da.

The Homogeneous MassExtend procedure, consisting of amplification, cleanup, and extension reactions, was done according to the manufacturer, with some modifications. Desalted PCR and extension oligonucleotides were obtained from Integrated DNA Technologies (Coralville, IA) and verified by MALDI-TOF mass spectrometry.

For the amplification reaction, the PCR cocktail was composed of 1x AmpliTaq buffer, 2.5 mmol/L MgCl₂, 115 mol/L deoxynucleotide triphosphates (Applied Biosystems, Foster City, CA), 3 to 5 ng DNA template, and 0.1 unit of AmpliTaq Gold DNA polymerase (Applied Biosystems). Forward and reverse primers were both at a 100 nmol/L final concentration in a total reaction volume of 6.6 µL. PCR and extension cycling was carried out in an MJ Research thermal cycler (Watertown, MA). PCR conditions included a 15-minute denaturation step at 95°C, followed by 44 cycles of 20 seconds at 95°C, 30 seconds at 62°C and 1 minute at 72°C, followed by a 3-minute hold at 72°C. Amplification was verified by agarose gel electrophoresis. Nonincorporated deoxynucleotide triphosphates were removed by incubating the remaining amplification product at 37°C for 20 minutes in the presence of 0.5 unit shrimp alkaline phosphatase (Sequenom), followed by 5 minutes at 85°C. Extension reactions were carried out by adding 1 to 0.6 mol/L extension primer, 0.5 unit Thermo Sequenase (Sequenom), and a dideoxy/deoxy nucleotide mixture of ddATP, ddCTP, dideoxythymidine 5'-triphosphate, and dGTP (Sequenom) at 50 mol/L each. The following cycling conditions were used: 2 minutes at 95°C, followed by 55 cycles of 5 seconds at 94°C, 5 seconds at 52°C, and 5 seconds at 72°C. Extension products were desalted with SpectroClean Resin (Sequenom). Sequenom 384-element Matrix preloaded Spectro chips were spotted with 15 nL of sample supernatant with a SpectroJet piezoelectric nanoplotter. MALDI-TOF mass spectrometry was carried out on a Bruker MALDI-TOF Biflex III instrument. Mass spectrometry and genotyping data acquisition were done using a Sequenom SpectroTYPER RT workstation.

The completion rate for genotyping was >98%. Reproducibility of genotyping in 80 duplicate samples from four subjects was >99.9%.

Statistical Analysis
Differences in means of selected characteristics between cases and controls were tested using t tests, using log-transformation where necessary to meet the normality assumption. Tests for Hardy-Weinberg equilibrium were done using the asymptotic Pearson's ² test. Unconditional logistic regression was used to generate odds ratios (ORs) and 95% confidence intervals (95% CIs) estimating the prostate cancer risk associated with DNA repair markers after adjusting for age and other factors including total caloric intake, waist-to-hip ratio, and insulin resistance (25). We also investigated potential combined effects of the DNA repair polymorphisms with other factors, including waist-to-hip ratio, insulin resistance, and intake of preserved foods and allium vegetables, on prostate cancer risk in this population (19-21), using cutoff levels defined by medians of the distribution of consumption among the control subjects. The significance of interaction terms representing the combined effects of other risk factors with DNA repair markers was tested using the likelihood ratio test (25). All reported P values are two-sided.

	Results

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Selected characteristics of cases and controls are shown in Table 1. Among cases, most tumors were moderately or poorly differentiated, with about two-thirds of the cases displaying clinically significant, advanced cancers in regional or remote stages. The mean waist-to-hip ratio and insulin resistance ratio differed significantly between cases and controls (P < 0.01).

	Discussion

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The XRCC1 gene product is involved in the base excision repair pathway, which corrects DNA damage primarily from ionizing radiation and alkylating agents (12, 26). Few studies have investigated the role of XRCC1 in prostate cancer. Previous studies in U.S. men have found nonsignificantly increased prostate cancer risks associated with the AA genotype (27, 28). Consistent with these previous observations, in this Shanghai population, we found a borderline significant independent risk increase associated with the XRCC1-399 AA genotype.

To our knowledge, no epidemiologic studies have investigated the role of MGMT-84 and prostate cancer risk. Our results suggest that the MGMT-84 T variant (the high-risk allele) may have a dominant effect, although we were unable to evaluate the effect of the TT genotype due to small numbers. We previously reported strong associations of abdominal obesity and insulin resistance with prostate cancer risk in this Shanghai population (19, 21, 29). In the current study, we show further that the excess prostate cancer risks associated with these risk factors are more pronounced among men carrying the variant allele of the MGMT-84 marker. Both obesity and insulin resistance are closely linked to chronic inflammation, which in turn can cause DNA damage (30, 31). The product of the MGMT gene (also known as the O⁶-alkylguanine-DNA alkyltransferase or AGT) operates through the direct DNA damage reversal pathway, repairing DNA damage caused by alkylating agents (14, 17), and is susceptible to inactivation or degradation by oxidative agents (32). In addition, hypermethylated MGMT can be found in prostate carcinomas and is believed to be involved in prostate carcinogenesis (33). Although of interest, the observed joint effects of MGMT-84 with insulin resistance need to be confirmed in larger studies.

The combined effect of the XRCC3-241 marker and intake of preserved foods was intriguing. Despite our observation of no independent effect of the XRCC3-241 polymorphism on prostate cancer risk, higher intake of preserved foods was associated with a modest 25% increase in prostate cancer risk among men with the CC genotype of the marker. In contrast, among men with the CT/TT genotypes, higher preserved food intake was associated with a markedly increased risk. Consumption of salted and preserved foods is relatively common in China and is a risk factor for prostate cancer in this study. These foods are abundant in nitrosamines and nitrosamine precursors, which are considered important food mutagens (34-36) and can transform adult human prostate epithelial cells (37). The XRCC3 gene product participates in DNA double-strand break/homologous recombination repair. In vitro studies suggest that homologous recombination repair enzymes, including the XRCC3 gene product, may be involved in resistance to alkylating DNA damage induced by nitrogen mustards (22, 23). The observed significant joint effects of preserved foods with the XRCC3-241 marker suggest a potential gene-environment effect that warrants further investigation.

Due to the small number of SNPs studied per gene in this investigation, it is possible that the observed associations are due to linkage disequilibrium of the studied loci with other nearby SNPs within the studied genes. Similarly, other genes, including those in other DNA damage repair pathways, may be related to the SNPs examined in this study and may have confounded the results. Expanded studies with large sample sizes and more comprehensive coverage of SNPs in these and other genes in the DNA repair pathways are needed to evaluate the effect of gene-gene and gene-environment interactions.

Survival and selection biases are minimal in this population-based study: Over 90% of the incident cases in Shanghai during the study period agreed to be interviewed for the study, and demographic and clinical factors did not differ between interviewed subjects who did and did not participate in the blood collection. In addition, misclassification of genotype is minimal in the study, as evidenced by the 99.9% concordance of genotyping results in 80 duplicate quality control samples. However, for certain markers, statistical power is limited due to the rarity of the variant alleles, and for that reason we cannot rule out the possibility of small-to-modest effects of these markers, particularly MGMT-143. Our assessment of SNP-covariate interactions in this study is limited by low statistical power (<50%). Therefore, we may have been unable to detect modest true interactions. Our results for interactions of DNA repair markers with other factors in this study should be considered merely suggestive, but they may serve to indicate new areas of research, particularly exposure-specific functional studies of these SNPs. Finally, because the population in Shanghai is ethnically homogeneous, our results may not be generalizable to other populations.

In summary, this population-based study conducted in a low-risk population suggests that the DNA repair polymorphisms, in particular XRCC1-399, XRCC3-241, and MGMT-84, may be associated with the risk of clinically significant prostate cancer in China. Our results also suggest that other risk factors, including preserved food intake, insulin resistance, and abdominal obesity, may operate in concert with genes in the DNA repair pathways to influence risk, although these findings from subgroup analyses should be considered suggestive and must be confirmed. Although we are unable to generalize our results directly to other populations, similar underlying biological mechanisms may exist for other racial/ethic groups. Larger studies are needed to confirm these results and clarify the mechanisms involved.

	Acknowledgments

 
We thank Jiaorong Cheng (Shanghai Cancer Institute) for specimen collection and processing, collaborating hospitals and urologists for data collection, and the pathologists for pathology review; Linda Lannom, John Heinrich, and Millie Bendel of Westat for study management and data preparation; Gigi Yuan (Information Management Systems, Inc.) for data management and analysis; Janis Koci (Scientific Applications International Corporation) for management of the biological samples; and the Advanced Technology Center of the National Cancer Institute for genotyping.

	Footnotes

 
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 11/ 5/04; revised 4/13/05; accepted 4/18/05.

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