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胚胎干细胞特异性基因的克隆:转录调控基因esg-1的特性分析

Cloning of embryonal stem cell-specific genes: characterization of the transcriptionally controlled gene esg-1.

作者信息

Bierbaum P, MacLean-Hunter S, Ehlert F, Möröy T, Müller R

机构信息

Institut für Molekularbiologie und Tumorforschung, Philipps-Universität Marburg, Germany.

出版信息

Cell Growth Differ. 1994 Jan;5(1):37-46.

PMID:8123591
Abstract

We have isolated, by differential library screening, eight cDNAs representing genes that are specifically expressed in the embryonal stem cell line IMT-11, when compared to the parietal endoderm-like cell line PYS-2 or to NIH3T3 fibroblasts. One of these genes, embryonal stem cell gene 1 (esg-1), was analyzed in detail. esg-1 mRNA is found at high levels in both IMT-11 and F9 embryonal carcinoma cells and disappears during the differentiation of the stem cells. Furthermore, expression of the gene was found to be extremely low in, or absent from, oocytes and fertilized eggs, but it is strongly induced at the 2-cell stage, reaching maximum levels at the 4-cell stage. In contrast, esg-1 expression is detectable neither in midgestation embryos nor in neonatal tissues. These results strongly suggest that esg-1 is expressed specifically or at least predominantly in embryonal stem cells. Antibodies directed against a glutathione S-transferase-esg-1 fusion product detect a protein of M(r) approximately 14,000 in F9 embryonal carcinoma cells, but not in differentiated cells. Apart from the esg-1 gene, which contains two introns, there are at least seven esg-1-related pseudogenes in the mouse genome that differ from the esg-1 gene by the presence of multiple point mutations, by the lack of intervening sequences, and/or by the presence of a polyadenylated stretch at the 3' end. The esg-1 gene is under stringent transcriptional control in differentiating and differentiated cells, as shown by both nuclear run-on assays and the transient F9 stem cell-specific expression of constructs consisting of esg-1 upstream sequences fused to a luciferase reporter gene.

摘要

通过差异文库筛选,我们分离出了8个cDNA,它们代表的基因在胚胎干细胞系IMT-11中特异性表达,与壁内胚层样细胞系PYS-2或NIH3T3成纤维细胞相比。其中一个基因,胚胎干细胞基因1(esg-1),得到了详细分析。esg-1 mRNA在IMT-11和F9胚胎癌细胞中均高水平存在,并在干细胞分化过程中消失。此外,该基因在卵母细胞和受精卵中的表达极低或不存在,但在2细胞期强烈诱导表达,在4细胞期达到最高水平。相反,在妊娠中期胚胎和新生组织中均未检测到esg-1表达。这些结果强烈表明esg-1在胚胎干细胞中特异性表达或至少主要表达。针对谷胱甘肽S-转移酶-esg-1融合产物的抗体在F9胚胎癌细胞中检测到一种分子量约为14,000的蛋白质,但在分化细胞中未检测到。除了包含两个内含子的esg-1基因外,小鼠基因组中至少有7个与esg-1相关的假基因,它们与esg-1基因的区别在于存在多个点突变、缺乏间隔序列和/或在3'端存在聚腺苷酸化延伸。如核转录分析和由esg-1上游序列与荧光素酶报告基因融合组成的构建体在F9干细胞中的瞬时特异性表达所示,esg-1基因在分化和已分化细胞中受到严格的转录调控。

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Cloning of embryonal stem cell-specific genes: characterization of the transcriptionally controlled gene esg-1.胚胎干细胞特异性基因的克隆:转录调控基因esg-1的特性分析
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