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亲环蛋白40(CyP-40),其hsp90结合结构域的定位以及FKBP52与CyP-40竞争hsp90结合的证据。

Cyclophilin 40 (CyP-40), mapping of its hsp90 binding domain and evidence that FKBP52 competes with CyP-40 for hsp90 binding.

作者信息

Ratajczak T, Carrello A

机构信息

Department of Endocrinology and Diabetes, Sir Charles Gairdner Hospital, Nedlands, 6009 Western Australia.

出版信息

J Biol Chem. 1996 Feb 9;271(6):2961-5. doi: 10.1074/jbc.271.6.2961.

DOI:10.1074/jbc.271.6.2961
PMID:8621687
Abstract

The structurally related immunophilins cyclophilin 40 (CyP-40) and FKBP52 have been identified as components of the unactivated estrogen receptor. Both immunophilins have a similar molecular architecture that includes a C-terminal segment with a tetratricopeptide repeat (TPR) domain predicted to mediate protein interaction. hsp90 is a common cellular target for CyP-40 and FKBP52. Deletion mutants of CyP-40 fused to glutathione S-transferase were immobilized on glutathione-agarose and then used in a rapid hsp90 retention assay to define regions of the CyP-40 C terminus that are important for hsp90 binding. Our evidence suggests that the TPR domain is not sufficient for stable association of CyP-40 with hsp90 and requires the participation of flanking acidic and basic residues clustered at the N- and C-terminal ends, respectively. Both microdomains are characterized by alpha-helical structures with segregated hydrophobic and charged residues. Corresponding regions were identified in FKBP52. By preincubating myometrial cytosol with lysates containing bacterially expressed FKBP52, we have shown that FKBP52 competes with CyP-40 for hsp90 binding. Our results raise the possibility of a mutually exclusive association of CyP-40 and FKBP52 with hsp90. This would lead to separate immunophilin-hsp90-receptor complexes and place the estrogen receptor under the control of distinct immunophilin signaling pathways.

摘要

结构相关的亲免蛋白亲环素40(CyP-40)和FKBP52已被鉴定为未活化雌激素受体的组成成分。这两种亲免蛋白具有相似的分子结构,包括一个C末端片段,该片段带有一个预测可介导蛋白质相互作用的四肽重复(TPR)结构域。热休克蛋白90(hsp90)是CyP-40和FKBP52共同的细胞靶点。将与谷胱甘肽S-转移酶融合的CyP-40缺失突变体固定在谷胱甘肽琼脂糖上,然后用于快速hsp90保留试验,以确定CyP-40 C末端中对hsp90结合重要的区域。我们的证据表明,TPR结构域不足以使CyP-40与hsp90稳定结合,还需要分别聚集在N末端和C末端的侧翼酸性和碱性残基的参与。这两个微结构域的特征都是具有分离的疏水和带电荷残基的α螺旋结构。在FKBP52中也鉴定出了相应区域。通过将子宫肌层细胞溶质与含有细菌表达的FKBP52的裂解物预孵育,我们发现FKBP52与CyP-40竞争hsp90结合。我们的结果提出了CyP-40和FKBP52与hsp90相互排斥结合的可能性。这将导致形成单独的亲免蛋白-hsp90-受体复合物,并使雌激素受体受不同亲免蛋白信号通路的控制。

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