An Beum-Soo, Kang Sung Keun, Shin Jae-Ho, Jeung Eui-Bae
Laboratory of Veterinary Biochemistry and Molecular Biology, College of Veterinary Medicine and Research Institute of Veterinary Medicine, Chungbuk National University, Cheongju, Chungbuk 361-763, Republic of Korea.
Mol Cell Endocrinol. 2002 Jun 14;191(2):177-86. doi: 10.1016/s0303-7207(02)00042-4.
Quantification of estrogen-induced changes in the expression levels of endogenous genes such as pS2 and vitellogenin could be an assay to detect estrogenicity of chemicals. Considering its regulation by estrogen, in the present study, we hypothesize that the calbindin-D(9k) (CaBP-9k) gene has the possibility as a biomarker for estrogenic response of the environmental estrogens. We analyzed the time- and dose-dependent CaBP-9k mRNA expression in the immature rats by 3-day injection of 17beta-estradiol (E2) and alkylphenol acid [octyl-phenol (OP) and nonylphenol (NP)] and bisphenol A(BPA)) which are environmentally persistent and reported to have some estrogenic activity in experimental test systems. The expression of CaBP-9k mRNA was compared with uterotropic response of the compounds. A significant increase in CaBP-9k mRNA expression was observed when treated with 1000 mg/kg body weight (BW) per day of OP (18-fold versus control), NP (17-fold versus control) and BPA (6-fold versus control) for 3 days in dot blot assays. Using Northern blot analysis, a more dramatic increase of CaBP-9k mRNA expression was observed when treated with 1000 mg/kg BW per day of OP (132-fold versus control) and NP (113-fold versus control) for 3 days. Treatment with 10 and 100 mg/kg BW per day of NP and 100 mg/kg BW per day of OP for 3 days induced a small but significant increase in CaBP-9k mRNA expression. As expected, a single dose of E2 (40 microg/kg BW per day) for 3 days induced a significant increase in CaBP-9k mRNA expression as revealed by dot (15-fold versus control) or Northern blot assay (102-fold versus control). In a time response experiment using Northern blot assay, a significant increase in CaBP-9k mRNA expression was observed as early as 3 h, peaked at 6 h and continued until 72 h after treatment with 1000 mg/kg BW per day of OP, NP, and 48 h after treatment with 1000 mg/kg BW per day of BPA. A similar time-dependent response was observed when assessed by dot blot assay. Uterotropic response of the compounds was determined and compared with CaBP-9k mRNA expression. The alkylphenolic compounds induced a significant increase in the uterine wet weight at 1000 mg/kg BW per day of OP and NP, not BPA. A strong correlation between in vivo uterotropic assay and CaBP-9k mRNA expression assay was observed. In order to investigate the possible mechanisms by which the compounds regulate CaBP-9k mRNA expression, we studied the effect of the compound on the ERalpha mRNA level using total RNA from the treated rats. The alkylphenolic compounds as well as E2 stimulate the expression of ERalpha mRNA in a similar pattern to that of CaBP-9k mRNA in terms of dose- and time-dependent response. Strong regulation of CaBP-9k mRNA expression by E2 and the environmental estrogens and its correlation with in vivo uterotropic assay suggest that CaBP-9k gene can be used as a biomarker gene for assaying estrogenicity of putative estrogenic compounds.
对诸如pS2和卵黄蛋白原等内源性基因表达水平的雌激素诱导变化进行定量分析,可能是一种检测化学物质雌激素活性的方法。考虑到其受雌激素的调控,在本研究中,我们假设钙结合蛋白-D(9k)(CaBP-9k)基因有可能作为环境雌激素雌激素反应的生物标志物。我们通过对未成熟大鼠连续3天注射17β-雌二醇(E2)、烷基酚酸[辛基酚(OP)和壬基酚(NP)]以及双酚A(BPA),分析了CaBP-9k mRNA表达的时间和剂量依赖性,这些物质在环境中具有持久性,并且在实验测试系统中据报道具有一定的雌激素活性。将CaBP-9k mRNA的表达与这些化合物的子宫增重反应进行了比较。在斑点印迹分析中,当每天以1000mg/kg体重(BW)的剂量处理OP(相对于对照组增加18倍)、NP(相对于对照组增加17倍)和BPA(相对于对照组增加6倍)3天时,观察到CaBP-9k mRNA表达显著增加。使用Northern印迹分析,当每天以1000mg/kg BW的剂量处理OP(相对于对照组增加132倍)和NP(相对于对照组增加113倍)3天时,观察到CaBP-9k mRNA表达有更显著的增加。每天以10mg/kg BW和100mg/kg BW的剂量处理NP以及每天以100mg/kg BW的剂量处理OP 3天,诱导CaBP-9k mRNA表达有小幅但显著的增加。正如预期的那样,连续3天每天单剂量注射E2(40μg/kg BW),通过斑点印迹分析(相对于对照组增加15倍)或Northern印迹分析(相对于对照组增加102倍)显示CaBP-9k mRNA表达显著增加。在使用Northern印迹分析的时间反应实验中,每天以1000mg/kg BW的剂量处理OP、NP后,早在3小时就观察到CaBP-9k mRNA表达显著增加,在6小时达到峰值,并持续到72小时;每天以1000mg/kg BW的剂量处理BPA后,在48小时观察到CaBP-9k mRNA表达显著增加。通过斑点印迹分析评估时也观察到类似的时间依赖性反应。测定了这些化合物的子宫增重反应,并与CaBP-9k mRNA表达进行比较。烷基酚类化合物在每天以1000mg/kg BW的剂量处理OP和NP时,而非BPA,诱导子宫湿重显著增加。观察到体内子宫增重试验与CaBP-9k mRNA表达试验之间有很强的相关性。为了研究这些化合物调节CaBP-9k mRNA表达的可能机制,我们使用处理后大鼠的总RNA研究了化合物对ERα mRNA水平的影响。烷基酚类化合物以及E2在剂量和时间依赖性反应方面,以与CaBP-9k mRNA相似的模式刺激ERα mRNA的表达。E2和环境雌激素对CaBP-9k mRNA表达的强烈调节及其与体内子宫增重试验的相关性表明,CaBP-9k基因可作为检测假定雌激素化合物雌激素活性的生物标志物基因。
