Ramamoorthy K, Wang F, Chen I C, Norris J D, McDonnell D P, Leonard L S, Gaido K W, Bocchinfuso W P, Korach K S, Safe S
Veterinary Physiology and Pharmacology, Texas A&M University, College Station 77843-4466, USA.
Endocrinology. 1997 Apr;138(4):1520-7. doi: 10.1210/endo.138.4.5056.
The estrogenic activity of dieldrin, toxaphene, and an equimolar mixture of both compounds (dieldrin/toxaphene) was investigated in the 21-day-old B6C3F1 mouse uterus, MCF-7 human breast cancer cells, and in yeast-based reporter gene assays. Treatment of the animals with 17beta-estradiol (E2) (0.0053 kg/day x3) resulted in a 3.1-, 4.8-, and 7.8-fold increase in uterine wet weight, peroxidase activity, and progesterone receptor binding, respectively. In contrast, treatment with 2.5, 15 and 60 micromol/kg (x3) doses of toxaphene, dieldrin, or dieldrin/toxaphene (equimolar) did not significantly induce a dose-dependent increase in any of the E2-induced responses. The organochlorine pesticides alone and the binary mixture did not bind to the mouse uterine estrogen receptor (ER) in a competitive binding assay using [3H]E2 as the radioligand. In parallel studies, estrogenic activities were determined in MCF-7 cells by using a cell proliferation assay and by determining induction of chloramphenicol acetyl transferase (CAT) activity in MCF-7 cells transiently transfected with plasmids containing estrogen-responsive 5'-promoter regions from the rat creatine kinase B and human cathepsin D genes. E2 caused a 24-fold increase in CAT activity in MCF-7 cells transiently transfected with creatine kinase B and a 3.8-fold increase in cells transiently transfected with the human cathepsin D construct. Treatment of MCF-7 cells with dieldrin, toxaphene, or an equimolar mixture of dieldrin plus toxaphene (10(-8)-10(-5) M) did not significantly induce cell proliferation or CAT activity in the transient transfection experiment with both plasmids. The relative competitive binding of the organochlorine pesticides was determined by incubating MCF-7 cells with 10(-9) M [3H]E2 in the presence or absence of 2 x 10(-7) M unlabeled E2 (to determine nonspecific binding), toxaphene (10(-5) M), dieldrin (10(-5) M), and equimolar concentrations of the dieldrin plus toxaphene mixture (10(-5) M). The binding observed for [3H]E2 in the whole cell extracts was displaced by unlabeled E2, whereas the organochlorine pesticides and binary mixture exhibited minimal to nondetectable competitive binding activity. E2 caused a 5000-fold induction of beta-galactosidase (beta-gal) activity in yeast transformed with the human ER and a double estrogen responsive element upstream of the beta-gal reporter gene. Treatment with 10(-6)-10(-4) M chlordane, dieldrin, toxaphene, or an equimolar mixture of dieldrin/toxaphene did not induce activity, whereas 10(-4) M endosulfan caused a 2000-fold increase in beta-gal activity. Diethylstilbestrol caused a 20-fold increase in activity in yeast transformed with the mouse ER and a single estrogen responsive element upstream of the beta-gal reporter gene. Dieldrin, chlordane, toxaphene, and endosulfan induced a 1.5- to 4-fold increase in activity at a concentration of 2.5 x 10(-5) M. Synergistic transactivation was not observed for any equimolar binary mixture of the pesticides at concentrations of either 2.5 x 10(-5) M or 2.5 x 10(-4) M. The results of this study demonstrate that for several estrogen-responsive assays in the mouse uterus, MCF-7 human breast cancer cells, and yeast-based reporter gene assays, the activities of both dieldrin and toxaphene were minimal, and no synergistic interactions were observed with a binary mixture of the two compounds.
在21日龄的B6C3F1小鼠子宫、MCF-7人乳腺癌细胞以及基于酵母的报告基因检测中,研究了狄氏剂、毒杀芬以及这两种化合物的等摩尔混合物(狄氏剂/毒杀芬)的雌激素活性。用17β-雌二醇(E2)(0.0053 kg/天×3)处理动物,导致子宫湿重、过氧化物酶活性和孕酮受体结合分别增加3.1倍、4.8倍和7.8倍。相比之下,用2.5、15和60 μmol/kg(×3)剂量的毒杀芬、狄氏剂或狄氏剂/毒杀芬(等摩尔)处理,并未显著诱导E2诱导反应中的任何一种出现剂量依赖性增加。在使用[3H]E2作为放射性配体的竞争性结合试验中,单独的有机氯农药及其二元混合物均未与小鼠子宫雌激素受体(ER)结合。在平行研究中,通过细胞增殖试验以及测定用含有大鼠肌酸激酶B和人组织蛋白酶D基因雌激素反应性5'-启动子区域的质粒瞬时转染的MCF-7细胞中氯霉素乙酰转移酶(CAT)活性,来测定MCF-7细胞中的雌激素活性。E2使瞬时转染肌酸激酶B的MCF-7细胞中的CAT活性增加24倍,使瞬时转染人组织蛋白酶D构建体的细胞中的CAT活性增加3.8倍。在用狄氏剂、毒杀芬或狄氏剂加毒杀芬的等摩尔混合物(10^(-8)-10^(-5) M)处理MCF-7细胞的瞬时转染实验中,用两种质粒处理均未显著诱导细胞增殖或CAT活性。通过在存在或不存在2×10^(-7) M未标记E2(以确定非特异性结合)、毒杀芬(10^(-5) M)、狄氏剂(10^(-5) M)以及狄氏剂加毒杀芬混合物的等摩尔浓度(10^(-5) M)的情况下,将MCF-7细胞与10^(-9) M [3H]E2孵育,来确定有机氯农药的相对竞争性结合。在全细胞提取物中观察到的[3H]E2结合被未标记的E2取代,而有机氯农药及其二元混合物表现出最小至无法检测到的竞争性结合活性。E2在用人类ER和β-半乳糖苷酶(β-gal)报告基因上游的双雌激素反应元件转化的酵母中,引起β-半乳糖苷酶活性5000倍的诱导。用10^(-6)-10^(-4) M氯丹、狄氏剂、毒杀芬或狄氏剂/毒杀芬的等摩尔混合物处理未诱导活性,而10^(-4) M硫丹使β-半乳糖苷酶活性增加2000倍。己烯雌酚在用小鼠ER和β-半乳糖苷酶报告基因上游的单个雌激素反应元件转化的酵母中使活性增加20倍。狄氏剂、氯丹、毒杀芬和硫丹在浓度为2.5×10^(-5) M时使活性增加1.5至4倍。在浓度为2.5×10^(-5) M或2.5×10^(-4) M时,未观察到任何农药等摩尔二元混合物的协同反式激活。本研究结果表明,在小鼠子宫、MCF-7人乳腺癌细胞以及基于酵母的报告基因检测中的几种雌激素反应性检测中,狄氏剂和毒杀芬的活性均最小,且未观察到这两种化合物的二元混合物具有协同相互作用。
