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γ射线诱导的染色体诱变敏感性与非裔美国女性患乳腺癌的风险相关:咖啡因可调节诱变敏感性检测的结果。

gamma-Radiation-induced chromosomal mutagen sensitivity is associated with breast cancer risk in African-American women: caffeine modulates the outcome of mutagen sensitivity assay.

作者信息

Natarajan Thanemozhi G, Ganesan Natarajan, Carter-Nolan Pamela, Tucker Cynthia A, Shields Peter G, Adams-Campbell Lucile L

机构信息

Medicine and Oncology, Lombardi Comprehensive Cancer Center, Georgetown University Medical Center, 3800 Reservoir Road, Northwest, LL (S) Level, Room 150, Box 571465, Washington, DC 20057-1465, USA.

出版信息

Cancer Epidemiol Biomarkers Prev. 2006 Mar;15(3):437-42. doi: 10.1158/1055-9965.EPI-05-0353.

Abstract

Several different cancer studies have indicated that lymphocyte mutagen sensitivity is a marker of DNA repair deficiency and increased cancer risk. We have used a mutagen sensitivity assay (MSA) measuring gamma-radiation-induced chromosomal aberrations in freshly cultured lymphocytes and assessed breast cancer risk in African-American women. Concurrently, we conducted duplicate cultures in the presence of caffeine, which overrides G(2) arrest in cultured cells, decreases time to DNA repair, and hence increases the aberration rate. In comparison with the non-caffeine-treated cells, we are conceptually segregating the contribution of DNA repair and time for DNA repair as individual susceptibility phenotypes. Blood samples were obtained from 61 cases and 86 controls at Howard University Hospital. Two sets of whole-blood cultures were established and gamma-irradiated (1 Gy) at 67 hours, one of which was treated with caffeine (1 mg/mL). Thereafter, cultures were processed for obtaining metaphase spreads. Fifty metaphases were screened for chromatid breaks. The mean breaks per cell (MBPC) for cases (0.34 +/- 0.15) was significantly greater than for controls (0.24 +/- 0.12; P < 0.0001). Using the 75th percentile value of controls as a cutoff to define mutagen sensitivity, the sensitive individuals had an odds ratio of 4.5 (95% confidence intervals, 2.2-9.1) for breast cancer compared with individuals that were not sensitive. The adjusted odds ratio was 3.3 (95% confidence intervals, 0.147-73.917), which was statistically significant but was limited by the small number of subjects. The results for caffeine co-culture were not predictive of breast cancer (MBPC: cases, 1.6 +/- 0.9 versus controls, 1.5 +/- 0.8; P = 0.8663). Comparing the MBPC for caffeine and non-caffeine cultures, there was a correlation in controls (n = 79; Spearman r = 0.4286; P < 0.0001), but not in cases (n = 58; Spearman r = 0.06609; P = 0.6221). This study indicates that the MSA phenotype is a risk factor for breast cancer in African-American women, with a significant effect observable even in small studies. The use of caffeine did not enhance the predictivity of MSA, but the correlation with non-caffeine cultures in controls indicates that the MSA phenotype is due to both DNA repair and G(2) arrest capacity.

摘要

多项不同的癌症研究表明,淋巴细胞诱变敏感性是DNA修复缺陷和癌症风险增加的一个标志。我们使用了一种诱变敏感性测定法(MSA),通过测量新鲜培养淋巴细胞中γ射线诱导的染色体畸变来评估非裔美国女性患乳腺癌的风险。同时,我们在咖啡因存在的情况下进行了重复培养,咖啡因会消除培养细胞中的G(2)期阻滞,缩短DNA修复时间,从而提高畸变率。与未用咖啡因处理的细胞相比,我们从概念上区分了DNA修复的作用和DNA修复时间,将其作为个体易感性表型。从霍华德大学医院的61例病例和86例对照中采集了血样。建立了两组全血培养物,并在67小时时进行γ射线照射(1 Gy),其中一组用咖啡因(1 mg/mL)处理。此后,对培养物进行处理以获得中期分裂相。筛选50个中期分裂相的染色单体断裂情况。病例组的平均每细胞断裂数(MBPC)为(0.34±0.15),显著高于对照组(0.24±0.12;P<0.0001)。以对照组的第75百分位数作为定义诱变敏感性的临界值,与不敏感个体相比,敏感个体患乳腺癌的优势比为4.5(95%置信区间,2.2 - 9.1)。调整后的优势比为3.3(95%置信区间,0.147 - 73.917),具有统计学意义,但受样本量少的限制。咖啡因共培养的结果不能预测乳腺癌(MBPC:病例组为1.6±0.9,对照组为1.5±0.8;P = 0.8663)。比较咖啡因培养组和非咖啡因培养组的MBPC,对照组(n = 79;Spearman相关系数r = 0.4286;P<0.0001)存在相关性,但病例组(n = 58;Spearman相关系数r = 0.06609;P = 0.6221)不存在相关性。这项研究表明,MSA表型是非裔美国女性患乳腺癌的一个风险因素,并表明即使在小型研究中也能观察到显著影响。咖啡因的使用并未提高MSA的预测能力,但对照组中与非咖啡因培养组的相关性表明,MSA表型是由DNA修复和G(2)期阻滞能力共同导致的。

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