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合成类固醇RU 486对Cre重组酶活性的调控

Regulation of Cre recombinase activity by the synthetic steroid RU 486.

作者信息

Kellendonk C, Tronche F, Monaghan A P, Angrand P O, Stewart F, Schütz G

机构信息

Molecular Biology of the Cell 1, German Cancer Research Center, Heidelberg.

出版信息

Nucleic Acids Res. 1996 Apr 15;24(8):1404-11. doi: 10.1093/nar/24.8.1404.

Abstract

To create a strategy for inducible gene targeting we developed a Cre-lox recombination system which responds to the synthetic steroid RU 486. Several fusions between Cre recombinase and the hormone binding domain (HBD) of a mutated human progesterone receptor, which binds RU 486 but not progesterone, were constructed. When tested in transient expression assays recombination activities of all fusion proteins were responsive to RU 486, but not to the endogenous steroid progesterone. However, the observed induction of recombination activity by the synthetic steroid varied between the different fusion proteins. The fusion with the highest activity in the presence of RU 486 combined with low background activity in the absence of the steroid was tested after stable expression in fibroblast and embryonal stem (ES) cells. We could demonstrate that its recombination activity was highly dependent on RU 486. Since the RU 486 doses required to activate recombination were considerably lower than doses displaying anti-progesterone effects in mice, this system could be used as a valuable tool for inducible gene targeting.

摘要

为了创建一种诱导型基因靶向策略,我们开发了一种对合成类固醇RU 486有反应的Cre-lox重组系统。构建了几种Cre重组酶与突变型人孕酮受体的激素结合域(HBD)的融合体,该突变型人孕酮受体可结合RU 486但不结合孕酮。在瞬时表达试验中进行测试时,所有融合蛋白的重组活性对RU 486有反应,但对内源性类固醇孕酮无反应。然而,合成类固醇对重组活性的诱导作用在不同的融合蛋白之间有所不同。在成纤维细胞和胚胎干细胞中稳定表达后,测试了在存在RU 486时活性最高且在不存在类固醇时背景活性较低的融合体。我们可以证明其重组活性高度依赖于RU 486。由于激活重组所需的RU 486剂量远低于在小鼠中显示抗孕酮作用的剂量,该系统可作为诱导型基因靶向的有价值工具。

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