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紧密的 Cosmc 伴侣蛋白与其特定的非天然 T-合成酶客户之间的复合物形成导致酶活性和客户驱动的解离。

Tight complex formation between Cosmc chaperone and its specific client non-native T-synthase leads to enzyme activity and client-driven dissociation.

机构信息

Department of Biochemistry, Emory University School of Medicine, Atlanta, Georgia 30322, USA.

出版信息

J Biol Chem. 2012 May 4;287(19):15317-29. doi: 10.1074/jbc.M111.312587. Epub 2012 Mar 13.

Abstract

The interaction of the endoplasmic reticulum molecular chaperone Cosmc with its specific client T-synthase (Core 1 β1-3-galactosyltransferase) is required for folding of the enzyme and eventual movement of the T-synthase to the Golgi, but the mechanism of interaction is unclear. Here we show that the lumenal domain of recombinant Cosmc directly interacts specifically in either free form or covalently bound to solid supports with denatured T-synthase but not with the active dimeric form of the enzyme. This leads to formation of a relatively stable complex of Cosmc and denatured T-synthase accompanied by formation of reactivated enzyme in an ATP-independent fashion that is not regulated by redox, calcium, pH, or intermolecular disulfide bond formation. The partly refolded and active T-synthase remains tightly bound noncovalently to Cosmc. Dissociation of T-synthase from the complex is promoted by further interactions of the complex with free forms of either native or non-native T-synthase. Taken together, these results demonstrate a novel mechanism in which Cosmc cycles to bind non-native T-synthase, leading to enzyme activity and release in a client-driven process.

摘要

内质网分子伴侣 Cosmc 与其特定的客户 T-合成酶(核心 1 β1-3-半乳糖基转移酶)的相互作用对于酶的折叠和 T-合成酶最终向高尔基体的移动是必需的,但相互作用的机制尚不清楚。在这里,我们表明重组 Cosmc 的腔域域以直接的方式特异性地与变性的 T-合成酶相互作用,无论是在游离形式还是共价结合到固体支持物上,而不是与酶的活性二聚体形式相互作用。这导致 Cosmc 和变性 T-合成酶形成相对稳定的复合物,伴随着以 ATP 非依赖性方式重新激活酶的形成,该过程不受氧化还原、钙、pH 或分子间二硫键形成的调节。部分重折叠和活性 T-合成酶仍然与 Cosmc 紧密非共价结合。进一步的复合物与游离的天然或非天然 T-合成酶相互作用,促进 T-合成酶从复合物中的解离。总之,这些结果表明了一种新的机制,其中 Cosmc 循环结合非天然 T-合成酶,导致在客户驱动的过程中释放具有酶活性的 T-合成酶。

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