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蜕皮激素受体和超气门蛋白的核定位与DNA结合

Nuclear localization and DNA binding of ecdysone receptor and ultraspiracle.

作者信息

Cronauer M V, Braun S, Tremmel Ch, Kröncke K-D, Spindler-Barth M

机构信息

Institute of General Zoology and Endocrinology, University of Ulm, Ulm, Germany.

出版信息

Arch Insect Biochem Physiol. 2007 Jul;65(3):125-33. doi: 10.1002/arch.20184.

Abstract

The Ecdysone receptor (EcR) is distributed between cytoplasm and nucleus in CHO cells. Nuclear localization is increased by the ligand Muristerone A. The most important heterodimerization partner Ultraspiracle (Usp) is localized predominantly in the nucleus. We used the diethylentriamine nitric oxide adduct DETA/NO, which releases NO and destroys the zinc-finger structure of nuclear receptors, to investigate whether nuclear EcR and Usp interact with DNA. If expressed separately, Usp and EcR in the absence of hormone do not interact with DNA. The hormone-induced increase in nuclear EcR is due to enhanced DNA binding. In the presence of Usp, EcR is shifted nearly quantitatively into the nucleus. Only a fraction (approximately 30%) of the heterodimer is sensitive to DETA/NO. Interaction of the heterodimer with DNA is mediated mainly by the C-domain of EcR. Deletion of the DNA-binding domain of Usp only slightly reduces nuclear localization of EcR/Usp, although the nuclear localization signal of Usp is not present anymore. The results indicate that EcR and Usp can enter the nucleus independently, but cotransport of both receptors mediated by dimerization via the ligand binding domains is possible even in the absence of hormone.

摘要

蜕皮激素受体(EcR)在CHO细胞的细胞质和细胞核之间分布。配体莫氏蜕皮素A可增加其核定位。最重要的异源二聚体伙伴超气门蛋白(Usp)主要定位于细胞核。我们使用二乙三胺一氧化氮加合物DETA/NO,其可释放NO并破坏核受体的锌指结构,以研究细胞核中的EcR和Usp是否与DNA相互作用。如果单独表达,在无激素的情况下,Usp和EcR不与DNA相互作用。激素诱导的细胞核EcR增加是由于DNA结合增强。在有Usp存在的情况下,EcR几乎定量地转移到细胞核中。只有一小部分(约30%)的异源二聚体对DETA/NO敏感。异源二聚体与DNA的相互作用主要由EcR的C结构域介导。删除Usp的DNA结合结构域只会略微降低EcR/Usp的核定位,尽管Usp的核定位信号已不复存在。结果表明,EcR和Usp可以独立进入细胞核,但即使在无激素的情况下,通过配体结合结构域二聚化介导的两种受体的共转运也是可能的。

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