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核定位和转录抑制局限于生物钟蛋白隐花色素中的可分离结构域。

Nuclear localization and transcriptional repression are confined to separable domains in the circadian protein CRYPTOCHROME.

作者信息

Zhu Haisun, Conte Francesca, Green Carla B

机构信息

Department of Biology, University of Virginia, Charlottesville, VA 22904, USA.

出版信息

Curr Biol. 2003 Sep 16;13(18):1653-8. doi: 10.1016/j.cub.2003.08.033.

DOI:10.1016/j.cub.2003.08.033
PMID:13678599
Abstract

Circadian rhythms are driven by molecular clocks composed of interlocking transcription/translation feedback loops. CRYPTOCHROME (CRY) proteins are critical components of these clocks and repress the activity of the transcription factor heterodimer CLOCK/BMAL1. Unlike the homologous DNA repair enzyme 6-4 PHOTOLYASE, CRYs have extended carboxyl-terminal tails and cannot repair DNA damage (reviewed in ). Unlike mammals, Xenopus laevis contains both CRYs (xCRYs) and 6-4 PHOTOLYASE (xPHOTOLYASE), providing an excellent comparative tool to study CRY repressive function. We can extend findings to CRYs in general because xCRYs share high sequence homology with mammalian CRYs. We show here that deletion of xCRYs' C-terminal domain produces proteins that are, like xPHOTOLYASE, unable to suppress CLOCK/BMAL1 activation. However, these truncations also cause the proteins to be cytoplasmically localized. A heterologous nuclear localization signal (NLS) restores the truncation mutants' nuclear localization and repressive activity. Our results demonstrate that the CRYs' C termini are essential for nuclear localization but not necessary for the suppression of CLOCK/BMAL1 activation; this finding indicates that these two functions reside in separable domains. Furthermore, the functional differences between CRYs and PHOTOLYASE can be attributed to the few amino acid changes in the conserved portions of these proteins.

摘要

昼夜节律由相互连锁的转录/翻译反馈环组成的分子时钟驱动。隐花色素(CRY)蛋白是这些时钟的关键组成部分,可抑制转录因子异二聚体CLOCK/BMAL1的活性。与同源DNA修复酶6-4光解酶不同,CRYs具有延伸的羧基末端尾巴,无法修复DNA损伤(相关综述见 )。与哺乳动物不同,非洲爪蟾同时含有CRYs(xCRYs)和6-4光解酶(xPHOTOLYASE),这为研究CRY抑制功能提供了一个绝佳的比较工具。由于xCRYs与哺乳动物CRYs具有高度的序列同源性,我们可以将研究结果推广到一般的CRYs。我们在此表明,缺失xCRYs的C末端结构域会产生与xPHOTOLYASE一样无法抑制CLOCK/BMAL1激活的蛋白质。然而,这些截短突变也会导致蛋白质定位于细胞质中。一个异源核定位信号(NLS)可恢复截短突变体的核定位和抑制活性。我们的结果表明,CRYs的C末端对于核定位至关重要,但对于抑制CLOCK/BMAL1激活并非必需;这一发现表明这两种功能存在于可分离的结构域中。此外,CRYs和光解酶之间的功能差异可归因于这些蛋白质保守部分的少数氨基酸变化。

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