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作 者:康鲁东[1] 吴伟芳[1] 崔福爱[1] 王秀利[2] 胡晓燕[1] 孔峰[1]
机构地区:[1]山东大学医学院生化与分子生物学研究所,山东济南250012 [2]郑州大学一附院骨科,河南郑州450052
出 处:《中国病理生理杂志》2007年第1期120-123,共4页Chinese Journal of Pathophysiology
基 金:山东省卫生厅基金资助项目(No.2003HZ042)
摘 要:目的:构建前列腺特异性表达的人前列腺特异膜抗原(PSMA)基因启动子/增强子表达载体,并进行组织特异性鉴定。方法:从人外周血中提取基因组DNA,采用PCR技术分别扩增PSMA上游1175bp的启动子序列,及第三内含子中258bp的增强子序列,将两个序列定向克隆至荧光素酶报告基因表达质粒pGL3-Basic,构建前列腺特异性表达载体pGL3-PSMP-PSME。将构建载体用脂质体分别转染前列腺癌PC-3M细胞株及4种非前列腺癌细胞株,48h后通过检测荧光素酶表达活性,确定克隆的启动子及增强子的活性及其组织特异性表达活性。结果:构建的pGL3-PSMP-PSME质粒经酶切及DNA测序分析鉴定,证实克隆片段的大小、插入方向及其序列正确。细胞转染结果显示,pGL3-PSMP-PSME在PC-3M细胞株中表达活性明显高于其它4种非前列腺癌细胞株。结论:构建的前列腺表达载体具有较高的组织特异性,为进一步研究PSMA调控序列驱动治疗基因进行前列腺癌的靶向生物治疗奠定了基础。To construct a prostate - specific expression vector of promoter and enhancer of human prostate -specific membrane antigen (PSMA). METHODS: The promoter and enhancer of PSMA were amplified by PCR separately. The two segments were cloned into the expression vector pGL3 - Basic, a prostate - specific expression vector pGL3 -PSMP -PSME was constructed. The vector was transfected into prostatic carcinoma cell PC -3M and four kinds of non - prostatic carcinoma cells by lipofectamine. The activity of luciferase of transfected cells and tissue specificity of vector was examined at 48 hours after transfection. RESULTS: With DNA sequence of the vector pGL3 - PSMP - PSME, the segment of clone was proved correct. The activity of luciferase of the pGL3 - PSMP - PSME was expressed distinctly in PC - 3 M and was not expressed in other nonprostate cell lines. CONCLUSION: The prostate- specific expression vector was constructed successfully. It lays foundation for studying target gene therapy of the prostate cancer.
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