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作 者:杨红斌[1] 付京[2] 张盈华[1] 郝新保[1] 邱福海[2] 张利朝[1]
机构地区:[1]第四军医大学唐都医院中心实验室,西安市710038 [2]第四军医大学唐都医院,西安市710038
出 处:《中国肿瘤临床》1999年第10期743-746,共4页Chinese Journal of Clinical Oncology
基 金:国家自然科学基金!资助(39380006)
摘 要:目的:观察36 例(E2 + ) 乳腺癌患者组织PR 和ER DNA 结合功能的关系,进而探讨(E2 + /PR+ ) 表型内分泌治疗无反应的分子机制。方法:用激素结合法和迁移率改变法。结果:1) 用含有ER 的MCF- 7 细胞株作为阳性对照,22 ℃Mg2 + 存在条件下,迁移率改变法中ER- ERE 复合物的形成是激素依赖性的,证实了ER- ERE 复合物的特性。2) 激素结合法和迁移率改变法检测结果显示,36 例(E2 + ) 乳腺癌中有25 例相一致,其中两种方法都是阳性者(PR+ /ERE+ )17 例,都是阴性者(PR- /ERE- )8 例。3 例肿瘤,激素结合法阳性而迁移率改变法阴性(PR+ /ERE- ) 。8 例肿瘤,激素结合法阴性而迁移率改变法阳性(PR- /ERE+ ) 。结论:乳腺癌组织中依赖ER 的PR 表达还有其它途径(PR+ /ERE- ) ,且PR 阴性不能表示ER DNA 结合功能状态有缺陷(PR- /ERE+ ) ,利用PR 评估ER DNA 结合功能状态以指导乳腺癌的内分泌治疗存在约30 % (11/36) 的误差率。因此,传统的激素结合法检测结果(E2 、PR) 同迁移率改变法检测结果(ERE) 相结合,能更准确地反应ERAim: To study the relationship between progesterone receptor (PR) and estrogen receptor (ER) DNA binding domain function in 36 breast cancers selected by testing E2 using hormone binding assay aiming to discuss the molecule mechanism of nonresponsiveness to endocrine therapy. Methods: Hormone binding assay and gel mobility shift assay were used. Results: 1)Using the ER-containing human breast cancer line MCF-7 as a positive control, we performed the mobility shift assay at 22℃in the presence of Mg2+to characterize the ER-ERE complex and found that the formation of ER-ERE complexes was estrogene-dependent. 2) Correlation of the mobility shift assay with the (PR )hormone-binding assay showed coincident with in 25 of the 36 tumors. Both assays were positive (PR+/ERE+) in 17 cases and both were negative in 8 cases. In 3 tumors, the hormone-binding assay was positive and the mobility shift assay negative (PR+/ERE-). In 8 cancers, the hormone-binding assay was negative and the mobility shift assay positive (PR-/ERE+). Conclusion: There is another pathway in the ER-dependent expression of PR in breast cancers and it is shown that PR(-) does not represent the defectiveness of ER DNA binding domain function, so there exist an 30% (11 / 36) error rate in the endocrine therapy according to PR estimation of the ER DNA binding domain function. Therefore, combination of detecting ERE (by the mobility shift assay) and PR (by hormone binding assay) could further truly determine the ER DNA binding domain function which could provide even more credible supports for postoperative aid endocrine therapy for breast cancers.
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