| Literature DB >> 17213827 |
J Kotsopoulos1, Z Chen, K A Vallis, A Poll, P Ainsworth, S A Narod.
Abstract
The BRCA1 gene product helps to maintain genomic integrity through its participation in the cellular response to DNA damage: specifically, the repair of double-stranded DNA breaks. An impaired cellular response to DNA damage is a plausible mechanism whereby BRCA1 mutation carriers are at increased risk of breast cancer. Hence, an individual's capacity to repair DNA may serve as a useful biomarker of breast cancer risk. The overall aim of the current study was to identify a biomarker of DNA repair capacity that could distinguish between BRCA1 mutation carriers and non-carriers. DNA repair capacity was assessed using three validated assays: the single-cell alkaline gel electrophoresis (comet) assay, the micronucleus test, and the enumeration of gamma-H2AX nuclear foci. DNA repair capacity of peripheral blood lymphocytes from 25 cancer-free female heterozygous BRCA1 mutation carriers and 25 non-carrier controls was assessed at baseline and following cell exposure to gamma-irradiation (2 Gy). We found no significant differences in the mean tail moment, in the number of micronuclei or in the number of gamma-H2AX nuclear foci between the carriers and non-carriers at baseline, and following gamma-irradiation. These data suggest that these assays are not likely to be useful in the identification of women at a high risk for breast cancer.Entities:
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Year: 2007 PMID: 17213827 PMCID: PMC2360222 DOI: 10.1038/sj.bjc.6603528
Source DB: PubMed Journal: Br J Cancer ISSN: 0007-0920 Impact factor: 7.640
Principal characteristics of the study participants, by mutation status
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| Age at interview (years), mean (s.d.) | 43.56 (9.81) | 44.62 (11.19) | 0.738 |
| Age at menarche, mean (s.d.) | 12.31 (1.40) | 12.36 (1.70) | 0.916 |
| Age at first birth, mean (s.d.) | 26.50 (5.00) | 26.79 (4.80) | 0.873 |
| Height (inches), mean (s.d.) | 64.38 (2.52) | 64.02 (2.15) | 0.589 |
| Weight (pounds), mean (s.d.) | 147.84 (30.46) | 154.04 (34.77) | 0.506 |
| BMI (kg m−2), mean (s.d.) | 25.02 (4.70) | 26.36 (5.63) | 0.367 |
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| Premenopausal | 10 (40) | 17 (68) | |
| Postmenopausal | 15 (60) | 8 (32) | 0.047 |
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| Non-user | 21 (84) | 25 (100) | |
| User | 4 (16) | 0 (0) | 0.037 |
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| Non-user | 23 (92) | 20 (80) | |
| User | 2 (8) | 5 (20) | 0.221 |
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| Non-user | 25 (100) | 22 (88) | |
| User | 0 (0) | 3 (12) | 0.074 |
| Total alcoholic drinks per day, mean (s.d.) | 0.73 (1.57) | 0.70 (0.69) | 0.935 |
| Energy intake (kcal day−1), mean (s.d.) | 1730.09 (540.23) | 1718.02 (443.41) | 0.934 |
| Total hours of physical activity per week, mean (s.d.) | 19.03 (7.25) | 22.60 (5.17) | 0.065 |
All P-values are univariate and were derived using the Student's t-test for continuous variables and the chi-square test for categorical variables.
s.d.=standard deviation.
Among parous women.
Current use.
Crude and adjusted mean tail moments in study population, stratified by BRCA1 mutation status
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| 0 | 0 | 2.63 (0.31) | 2.80 (0.31) | 0.696 | 2.99 (0.31) | 2.74 (0.15) | 0.472 |
| 2 | 0 | 7.99 (0.67) | 7.96 (0.66) | 0.974 | 8.37 (0.59) | 7.90 (0.32) | 0.486 |
| 2 | 1 | 3.64 (0.44) | 3.71 (0.38) | 0.907 | 4.05 (0.41) | 3.68 (0.17) | 0.396 |
The Student's t-test used to test for differences in the crude and adjusted means of the tail moments between BRCA1 mutation carriers and non-carriers.
Multivariate linear regression included terms for age (years), BMI (kg m−2), current smoker (yes/no), alcohol intake (total drinks of per day), physical activity (total hours of per week), and total daily caloric intake (kcal).
Figure 1Distribution of radiation-induced mean tail moments in the entire study population. Shaded boxes represent women who are BRCA1 and the black boxes represent women who are BRCA1. The solid vertical line represents the cutoff point between radiosensitive and non-sensitive individuals and was based on the 90th percentile of the non-carrier population after 2 Gy of γ-irradiation and one hour of recovery time (cutoff=6.39).
Crude and adjusted mean micronucleus frequencies, stratified by BRCA1 mutation carriers and non-carriers
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| 0 | 0 | 25.06 (3.39) | 18.00 (2.89) | 0.120 | 20.89 (3.26) | 19.96 (1.81) | 0.794 |
| 2 | 0 | 132.77 (12.39) | 128.84 (12.03) | 0.821 | 124.70 (4.69) | 139.79 (7.37) | 0.114 |
The Student's t-test used to test for differences in the crude and adjusted means of the tail moments between BRCA1 mutation carriers and non-carriers.
Multivariate linear regression included terms for age (years), BMI (kg m−2), current smoker (yes/no), alcohol intake (total drinks of per day), physical activity (total hours per week), and total daily caloric intake (kcal).
Figure 2Distribution of radiation-induced micronucleus frequencies in the entire study population. Shaded boxes represent women who are BRCA1 and the black boxes represent women who are BRCA1. The solid vertical line represents the cutoff point between radiosensitive and non-sensitive individuals and was based on the 90th percentile of the non-carrier population after 2 Gy of γ-irradiation and no recovery time (cutoff=197.69).
Crude and adjusted mean γ-H2AX foci in study population, stratified by BRCA1 mutation status
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| 0 | 0 h | 11.74 (4.63) | 8.78 (3.03) | 0.621 | 9.46 (4.23) | 11.67 (1.77) | 0.641 |
| 2 | 30 min | 30.14 (4.50) | 25.68 (2.93) | 0.447 | 25.00 (5.31) | 31.18 (2.47) | 0.323 |
| 2 | 3 h | 31.17 (4.79) | 32.31 (4.39) | 0.864 | 25.77 (4.89) | 33.24 (3.68) | 0.229 |
The Student's t-test used to test for differences in the crude and adjusted means of the tail moments between BRCA1 mutation carriers and non-carriers.
Multivariate linear regression included terms for age (years), BMI (kg m−2), current smoker (yes/no), alcohol intake (total drinks of per day), physical activity (total hours per week), and total daily caloric intake (kcal).
Figure 3Distribution of radiation-induced γ-H2AX foci in the entire study population. Shaded boxes represent women who are BRCA1 and the black boxes represent women who are BRCA1. The solid vertical line represents the cutoff point between radiosensitive and non-sensitive individuals and was based on the 90th percentile of the non-carrier population after 2 Gy of γ-irradiation and 3 h of recovery time (cutoff=62.01).