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用于测量染料木黄酮对乳腺癌发生影响的重水标记法。

Heavy water labeling method for measuring the effect of genistein on mammary gland carcinogenesis.

作者信息

Kim Hyeon-A, Jeong Kyu-Shik, Park Dae-Hun, Lee Jeong-Ae, Jeong Won-Il, Kim Yoo Kyeong

机构信息

Major in Food & Nutrition, Mokpo National University, Mokpo, Korea.

出版信息

Mol Cell Biochem. 2007 Jul;301(1-2):201-8. doi: 10.1007/s11010-007-9412-y. Epub 2007 Feb 21.

Abstract

Heavy water labeling method was applied to measure the effect of genistein on mammary gland carcinogenesis by incoporating (2)H from (2)H(2)O into the deoxyribose (dR) moiety of purine deoxyribonucleotides in dividing cells. In the present study, we followed the study design of Lamartiniere group to evaluate the efficacy of (2)H(2)O labeling on the measurement of mammary gland carconogenesis. Female Sprague-Dawley rats were fed estrogen-free AIN-93G diet starting 1 week before breeding and continuing through pregnancy and lactation. Female pups were assigned to the following groups on postnatal day 16 and fed AIN-93G diet: vehicle (dimethylsulfoxide) (DMSO), genistein, and estradiol benzoate (EB). On postnatal days 16, 18, and 20, female pups were injected subcutaneously with 500 mug genistein/g body wt, 500 ng EB/g body wt, or an equivalent volume of the vehicle. At day 50 postpartum, half of each group were gavaged with 60 mg dimethylbenz[a]anthracene (DMBA) in perila oil. After 1 week of DMBA treatment, all animals were labeled with (2)H(2)O by administration of 4% (2)H(2)O in drinking water after single intraperitonial bolus injection with 99.9% (2)H(2)O until sacrifice on postnatal day 81. The time-dependent weight gains were observed in all groups throughout the experimental period. The enrichment of body (2)H(2)O was attained at 1.84-2.47% through oral administration of (2)H(2)O. Mammary epithelial cell proliferation was measured by enrichment (EM1) of dA from rats. DMBA-treated groups showed higher fractional synthesis than DMBA non-treated groups. The group exposed only to genistein showed significantly lower EM1 (1.46 +/- 0.87%) than those of control groups, i.e., the DMBA non-treated group (2.28 +/- 0.29%) and the DMBA-treated group (2.32 +/- 0.28%). Bromodeoxyuridine (BrdU) immunostaining of mammary tissue revealed that genistein reduced proliferation of the mammary epithelial, and the number of cells stained positive for BrdU both in DMBA-treated groups and DMBA non-treated groups. H&E staining of mammary epithelium also showed that the exposure to genistein decreased proliferation of the mammary epithelium. The epithelium in the rats treated with DMBA showed mostly multiple cell layers, in contrast to the mostly double layer shown in the DMBA non-treated rats. The exposure to genistein in the prepubertal period inhibited mammary epithelial cell proliferation. In conclusion, the (2)H(2)O labeling results were in good agreement with the results of BrdU incorporation and histomorphometry, which demonstrates that (2)H(2)O labeling can be used as a tool to measure carcinogenesis.

摘要

采用重水标记法,通过将(2)H2O中的(2)H掺入分裂细胞中嘌呤脱氧核糖核苷酸的脱氧核糖(dR)部分,来测定染料木黄酮对乳腺癌发生的影响。在本研究中,我们遵循拉马蒂尼埃小组的研究设计,评估(2)H2O标记在测量乳腺癌发生方面的效果。雌性斯普拉格-道利大鼠在繁殖前1周开始喂食不含雌激素的AIN-93G饮食,并持续整个怀孕和哺乳期。雌性幼崽在出生后第16天被分配到以下组,并喂食AIN-93G饮食:溶剂对照组(二甲基亚砜)(DMSO)、染料木黄酮组和苯甲酸雌二醇(EB)组。在出生后第16、18和20天,雌性幼崽皮下注射500μg染料木黄酮/克体重、500ng EB/克体重或等量的溶剂。在产后第50天,每组的一半动物用紫苏油中的60mg二甲基苯并[a]蒽(DMBA)灌胃。DMBA处理1周后,在单次腹腔推注99.9%(2)H2O后,通过在饮用水中给予4%(2)H2O对所有动物进行(2)H2O标记,直至在出生后第81天处死。在整个实验期间观察到所有组的体重随时间增加。通过口服(2)H2O,体内(2)H2O的富集达到1.84 - 2.47%。通过测量大鼠dA的富集(EM1)来检测乳腺上皮细胞增殖。DMBA处理组的合成分数高于未处理组。仅暴露于染料木黄酮的组显示出显著低于对照组的EM1(1.46±0.87%),即未处理DMBA组(2.28±0.29%)和处理DMBA组(2.32±0.28%)。乳腺组织的溴脱氧尿苷(BrdU)免疫染色显示,染料木黄酮在DMBA处理组和未处理组中均降低了乳腺上皮细胞的增殖以及BrdU染色阳性的细胞数量。乳腺上皮的苏木精-伊红(H&E)染色也显示,暴露于染料木黄酮会降低乳腺上皮细胞的增殖。与未处理DMBA的大鼠大多为双层上皮相比,用DMBA处理的大鼠上皮大多为多层细胞。青春期前暴露于染料木黄酮可抑制乳腺上皮细胞增殖。总之,(2)H2O标记结果与BrdU掺入和组织形态计量学结果高度一致,这表明(2)H2O标记可作为一种测量癌症发生的工具。

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