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H-NOX 激活的分子机制的结构见解。

Structural insights into the molecular mechanism of H-NOX activation.

机构信息

Department of Molecular and Cell Biology, University of California, Berkeley, California 94720, USA.

出版信息

Protein Sci. 2010 Apr;19(4):881-7. doi: 10.1002/pro.357.

Abstract

Nitric oxide (NO) signaling in mammals controls important processes such as smooth muscle relaxation and neurotransmission by the activation of soluble guanylate cyclase (sGC). NO binding to the heme domain of sGC leads to dissociation of the iron-histidine (Fe-His) bond, which is required for enzyme activity. The heme domain of sGC belongs to a larger class of proteins called H-NOX (Heme-Nitric oxide/OXygen) binding domains. Previous crystallographic studies on H-NOX domains demonstrate a correlation between heme bending and protein conformation. It was unclear, however, whether these structural changes were important for signal transduction. Subsequent NMR solution structures of H-NOX proteins show a conformational change upon disconnection of the heme and proximal helix, similar to those observed in the crystallographic studies. The atomic details of these conformational changes, however, are lacking in the NMR structures especially at the heme pocket. Here, a high-resolution crystal structure of an H-NOX mutant mimicking a broken Fe-His bond is reported. This mutant exhibits specific changes in heme conformation and major N-terminal displacements relative to the wild-type H-NOX protein. Fe-His ligation is ubiquitous in all H-NOX domains, and therefore, the heme and protein conformational changes observed in this study are likely to occur throughout the H-NOX family when NO binding leads to rupture of the Fe-His bond.

摘要

哺乳动物中的一氧化氮(NO)信号通过激活可溶性鸟苷酸环化酶(sGC)来控制重要的过程,如平滑肌松弛和神经递质传递。NO 与 sGC 的血红素结构域结合会导致铁-组氨酸(Fe-His)键的解离,这是酶活性所必需的。sGC 的血红素结构域属于一类更大的蛋白质,称为 H-NOX(血红素-一氧化氮/氧)结合结构域。以前对 H-NOX 结构域的晶体学研究表明血红素弯曲与蛋白质构象之间存在相关性。然而,这些结构变化是否对信号转导很重要尚不清楚。随后对 H-NOX 蛋白的 NMR 溶液结构的研究表明,在血红素和近端螺旋断开时会发生构象变化,类似于在晶体学研究中观察到的变化。然而,这些构象变化的原子细节在 NMR 结构中缺乏,特别是在血红素口袋中。本文报道了一种模拟断裂的 Fe-His 键的 H-NOX 突变体的高分辨率晶体结构。与野生型 H-NOX 蛋白相比,该突变体的血红素构象和主要 N 端位移发生了特定变化。Fe-His 键的配位在所有 H-NOX 结构域中都是普遍存在的,因此,当 NO 结合导致 Fe-His 键断裂时,本研究中观察到的血红素和蛋白质构象变化可能会发生在整个 H-NOX 家族中。

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