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人类生物钟基因(CLOCK)的分子克隆与特性分析:视交叉上核中的表达

Molecular cloning and characterization of the human CLOCK gene: expression in the suprachiasmatic nuclei.

作者信息

Steeves T D, King D P, Zhao Y, Sangoram A M, Du F, Bowcock A M, Moore R Y, Takahashi J S

机构信息

Department of Neurobiology and Physiology, Howard Hughes Medical Institute, Northwestern University, 2153 North Campus Drive, Evanston, Illinois, 60208-3520, USA.

出版信息

Genomics. 1999 Apr 15;57(2):189-200. doi: 10.1006/geno.1998.5675.

DOI:10.1006/geno.1998.5675
PMID:10198158
Abstract

The Clock gene is an essential regulator of circadian rhythms. It encodes a member of the basic helix-loop-helix/PER-ARNT-SIM family of transcription factors known to play a central role in the control of diverse cellular events. Previously we described the functional identification and molecular isolation of the Clock gene in the mouse, its interaction with the BMAL1 protein, and the role of this complex as a transcriptional activator in the circadian pacemaker. Here, we report the cloning, exon organization, chromosomal location, and mRNA expression of the human CLOCK gene. The coding sequence of human CLOCK extends for 2538 bp and is 89% identical to its mouse ortholog; its deduced amino acid sequence is 846 residues long and is 96% identical to mouse CLOCK. Radiation hybrid mapping localized human CLOCK to the long arm of human chromosome 4 (4q12). Direct sequencing of a genomic CLOCK clone indicated that the coding sequence of human CLOCK extends over 20 exons and that its intron/exon organization is identical to that of the mouse ortholog. Northern blot analysis indicated widespread expression of two major transcripts of 8 and 10 kb, and in situ hybridization of human brain tissue revealed elevated expression of CLOCK mRNA in the suprachiasmatic nuclei, the locus of circadian control in mammals, and in the cerebellum. Comparison of cDNA clones revealed two single nucleotide polymorphisms in noncoding sequence flanking the CLOCK open reading frame. The central role of Clock in the organization of circadian rhythms suggests that it will be a useful candidate gene for genetic analyses of disorders associated with dysfunction of the circadian system.

摘要

Clock基因是昼夜节律的重要调节因子。它编码一种属于碱性螺旋-环-螺旋/PER-ARNT-SIM转录因子家族的成员,已知该家族在控制多种细胞事件中起核心作用。此前我们描述了小鼠中Clock基因的功能鉴定和分子分离、它与BMAL1蛋白的相互作用,以及该复合物作为昼夜节律起搏器中的转录激活因子的作用。在此,我们报告人类CLOCK基因的克隆、外显子组织、染色体定位和mRNA表达。人类CLOCK的编码序列延伸2538 bp,与其小鼠直系同源基因的序列一致性为89%;其推导的氨基酸序列长846个残基,与小鼠CLOCK的序列一致性为96%。辐射杂种图谱将人类CLOCK定位到人类染色体4的长臂(4q12)。对一个基因组CLOCK克隆的直接测序表明,人类CLOCK的编码序列跨越20个外显子,其内含子/外显子组织与小鼠直系同源基因相同。Northern印迹分析表明,有8 kb和10 kb两种主要转录本广泛表达,人脑组织的原位杂交显示,CLOCK mRNA在视交叉上核(哺乳动物昼夜节律控制的位点)和小脑中表达升高。cDNA克隆的比较揭示了CLOCK开放阅读框侧翼非编码序列中的两个单核苷酸多态性。Clock在昼夜节律组织中的核心作用表明,它将是对与昼夜节律系统功能障碍相关疾病进行遗传分析的一个有用候选基因。

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