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烟酰胺腺嘌呤二核苷酸磷酸(还原型)(NADP(H))传感器蛋白中二核苷酸结合折叠结构的重塑

Restructuring of the dinucleotide-binding fold in an NADP(H) sensor protein.

作者信息

Zheng Xiaofeng, Dai Xueyu, Zhao Yanmei, Chen Qiang, Lu Fei, Yao Deqiang, Yu Quan, Liu Xinping, Zhang Chuanmao, Gu Xiaocheng, Luo Ming

机构信息

National Laboratory of Protein Engineering and Plant Genetic Engineering, Department of Biochemistry and Molecular Biology, College of Life Sciences, Peking University, Beijing 100871, China.

出版信息

Proc Natl Acad Sci U S A. 2007 May 22;104(21):8809-14. doi: 10.1073/pnas.0700480104. Epub 2007 May 11.

Abstract

NAD(P) has long been known as an essential energy-carrying molecule in cells. Recent data, however, indicate that NAD(P) also plays critical signaling roles in regulating cellular functions. The crystal structure of a human protein, HSCARG, with functions previously unknown, has been determined to 2.4-A resolution. The structure reveals that HSCARG can form an asymmetrical dimer with one subunit occupied by one NADP molecule and the other empty. Restructuring of its NAD(P)-binding Rossmann fold upon NADP binding changes an extended loop to an alpha-helix to restore the integrity of the Rossmann fold. The previously unobserved restructuring suggests that HSCARG may assume a resting state when the level of NADP(H) is normal within the cell. When the NADP(H) level passes a threshold, an extensive restructuring of HSCARG would result in the activation of its regulatory functions. Immunofluorescent imaging shows that HSCARG redistributes from being associated with intermediate filaments in the resting state to being dispersed in the nucleus and the cytoplasm. The structural change of HSCARG upon NADP(H) binding could be a new regulatory mechanism that responds only to a significant change of NADP(H) levels. One of the functions regulated by HSCARG may be argininosuccinate synthetase that is involved in NO synthesis.

摘要

长期以来,人们一直认为NAD(P)是细胞中一种重要的能量携带分子。然而,最近的数据表明,NAD(P)在调节细胞功能方面也起着关键的信号传导作用。一种人类蛋白质HSCARG的晶体结构已被确定,分辨率为2.4埃,其功能此前未知。该结构表明,HSCARG可以形成一个不对称二聚体,其中一个亚基被一个NADP分子占据,另一个亚基为空。NADP结合后,其NAD(P)结合罗斯曼折叠的重组将一个延伸环转变为一个α螺旋,以恢复罗斯曼折叠的完整性。此前未观察到的重组表明,当细胞内NADP(H)水平正常时,HSCARG可能处于静止状态。当NADP(H)水平超过阈值时,HSCARG的广泛重组将导致其调节功能的激活。免疫荧光成像显示,HSCARG从静止状态下与中间丝相关联重新分布到分散在细胞核和细胞质中。NADP(H)结合后HSCARG的结构变化可能是一种仅对NADP(H)水平的显著变化做出反应的新调节机制。受HSCARG调节的功能之一可能是参与一氧化氮合成的精氨琥珀酸合成酶。

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