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比较功能基因组学揭示了isl1基因的三个增强子在运动和感觉神经元特异性表达方面的保守性和多样性。

Comparative functional genomics revealed conservation and diversification of three enhancers of the isl1 gene for motor and sensory neuron-specific expression.

作者信息

Uemura Osamu, Okada Yohei, Ando Hideki, Guedj Mickael, Higashijima Shin-Ichi, Shimazaki Takuya, Chino Naoichi, Okano Hideyuki, Okamoto Hitoshi

机构信息

Laboratory for Developmental Gene Regulation, Brain Science Institute, RIKEN, 2-1 Hirosawa, Wako, Saitama 351-0198, Japan.

出版信息

Dev Biol. 2005 Feb 15;278(2):587-606. doi: 10.1016/j.ydbio.2004.11.031.

DOI:10.1016/j.ydbio.2004.11.031
PMID:15680372
Abstract

Islet-1 (Isl1) is a member of the Isl1 family of LIM-homeodomain transcription factors (LIM-HD) that is expressed in a defined subset of motor and sensory neurons during vertebrate embryogenesis. To investigate how this specific expression of isl1 is regulated, we searched for enhancers of the isl1 gene that are conserved in vertebrate evolution. Initially, two enhancer elements, CREST1 and CREST2, were identified downstream of the isl1 locus in the genomes of fugu, chick, mouse, and human by BLAST searching for highly similar elements to those originally identified as motor and sensory neuron-specific enhancers in the zebrafish genome. The combined action of these elements is sufficient for completely recapitulating the subtype-specific expression of the isl1 gene in motor neurons of the mouse spinal cord. Furthermore, by direct comparison of the upstream flanking regions of the zebrafish and human isl1 genes, we identified another highly conserved noncoding element, CREST3, and subsequently C3R, a similar element to CREST3 with two CDP CR1 recognition motifs, in the upstream regions of all other isl1 family members. In mouse and human, CRESTs are located as far as more than 300 kb away from the isl1 locus, while they are much closer to the isl1 locus in zebrafish. Although all of zebrafish CREST2, CREST3, and C3R activate gene expression in the sensory neurons of zebrafish, CREST2 of mouse and human does not have the sequence necessary for sensory neuron-specific expression. Our results revealed both a remarkable conservation of the regulatory elements regulating subtype-specific gene expression in motor and sensory neurons and the dynamic process of reorganization of these elements whereby each element increases the level of cell-type specificity by losing redundant functions with the other elements during vertebrate evolution.

摘要

胰岛-1(Isl1)是LIM同源域转录因子(LIM-HD)的Isl1家族成员,在脊椎动物胚胎发育过程中,于特定的运动和感觉神经元亚群中表达。为了研究Isl1的这种特异性表达是如何调控的,我们寻找了在脊椎动物进化中保守的Isl1基因增强子。最初,通过BLAST搜索河豚、鸡、小鼠和人类基因组中Isl1基因座下游与最初在斑马鱼基因组中鉴定为运动和感觉神经元特异性增强子高度相似的元件,确定了两个增强子元件CREST1和CREST2。这些元件的联合作用足以完全重现Isl1基因在小鼠脊髓运动神经元中的亚型特异性表达。此外,通过直接比较斑马鱼和人类Isl1基因的上游侧翼区域,我们在所有其他Isl1家族成员的上游区域鉴定出另一个高度保守的非编码元件CREST3,随后又鉴定出C3R,它是与CREST3相似的元件,具有两个CDP CR1识别基序。在小鼠和人类中,CRESTs距离Isl1基因座超过300 kb,而在斑马鱼中它们距离Isl1基因座更近。尽管斑马鱼的所有CREST2、CREST3和C3R都能激活斑马鱼感觉神经元中的基因表达,但小鼠和人类的CREST2不具有感觉神经元特异性表达所需的序列。我们的结果揭示了在运动和感觉神经元中调控亚型特异性基因表达的调控元件的显著保守性,以及这些元件重新组织的动态过程,即每个元件在脊椎动物进化过程中通过与其他元件失去冗余功能来提高细胞类型特异性水平。

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