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在RB基因缺陷胚胎中异常表达的一个新基因的克隆与功能研究。

Cloning and functional studies of a novel gene aberrantly expressed in RB-deficient embryos.

作者信息

Yuan S S, Cox L A, Dasika G K, Lee E Y

机构信息

Department of Molecular Medicine/Institute of Biotechnology, University of Texas Health Science Center at San Antonio, San Antonio, Texas, 78245, USA.

出版信息

Dev Biol. 1999 Mar 1;207(1):62-75. doi: 10.1006/dbio.1998.9141.

DOI:10.1006/dbio.1998.9141
PMID:10049565
Abstract

The tumor suppressor RB regulates diverse cellular processes such as G1/S transition, cell differentiation, and cell survival. Indeed, Rb-knockout mice exhibit phenotypes including ectopic mitosis, defective differentiation, and extensive apoptosis in the neurons. Using differential display, a novel gene, Rig-1, was isolated based on its elevated expression in the hindbrain and spinal cord of Rb-knockout embryos. The longest open reading frame of Rig-1 encoded a polypeptide that consists of a putative extracellular segment with five immunoglobulin-like domains and three fibronectin III-like domains, a putative transmembrane domain, and a distinct intracellular segment. The Rig-1 sequence was 40% identical to the recently identified roundabout protein. Consistent with the predicted transmembrane nature of the protein, Rig-1 protein was present in the membranous fraction. Antisera raised against the putative extracellular and intracellular segments of Rig-1 reacted with an approximately 210-kDa protein in mouse embryonic CNS. Rig-1 mRNA was transiently expressed in the embryonic hindbrain and spinal cord. Elevated levels of Rig-1 mRNA and protein were found in Rb-/- embryos. Ectopic expression of a transmembrane form of Rig-1, but not the secreted form, promoted neuronal cell entrance to S phase and repressed the expression of a marker of differentiated neuron, Talpha1 tubulin. Thus Rig-1, a possible distant relative of roundabout, may mediate some of the pleiotropic roles of RB in the developing neurons.

摘要

肿瘤抑制因子RB调控多种细胞过程,如G1/S期转换、细胞分化和细胞存活。实际上,Rb基因敲除小鼠表现出包括异位有丝分裂、分化缺陷以及神经元广泛凋亡等表型。利用差异显示技术,基于其在Rb基因敲除胚胎的后脑和脊髓中表达升高,分离出一个新基因Rig-1。Rig-1最长的开放阅读框编码一种多肽,该多肽由一个具有五个免疫球蛋白样结构域和三个纤连蛋白III样结构域的假定细胞外区段、一个假定跨膜结构域以及一个独特的细胞内区段组成。Rig-1序列与最近鉴定出的robo蛋白有40%的同源性。与该蛋白预测的跨膜性质一致,Rig-1蛋白存在于膜组分中。针对Rig-1假定的细胞外和细胞内区段产生的抗血清与小鼠胚胎中枢神经系统中一种约210 kDa的蛋白发生反应。Rig-1 mRNA在胚胎后脑和脊髓中短暂表达。在Rb-/-胚胎中发现Rig-1 mRNA和蛋白水平升高。Rig-1跨膜形式而非分泌形式的异位表达促进神经元细胞进入S期,并抑制分化神经元标志物Talpha1微管蛋白的表达。因此,Rig-1作为robo的一个可能远亲,可能介导RB在发育中的神经元中的一些多效性作用。

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