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肥大细胞中白细胞介素-1受体相关T1基因的GATA依赖性表达。

GATA-Dependent expression of the interleukin-1 receptor-related T1 gene in mast cells.

作者信息

Gächter T, Moritz D R, Gheyselinck J, Klemenz R

机构信息

Division of Cancer Research, Department of Pathology, University Hospital, CH-8091 Zürich, Switzerland.

出版信息

Mol Cell Biol. 1998 Sep;18(9):5320-31. doi: 10.1128/MCB.18.9.5320.

Abstract

The murine delayed-early serum-responsive gene T1 encodes glycoproteins of the interleukin-1 receptor family. Transcriptional initiation in fibroblasts is regulated by c-Fos and gives rise to a rare 5-kb mRNA and an abundant 2.7-kb mRNA. These transcripts are translated into a receptor-like membrane-anchored protein and a secreted protein consisting only of the ectodomain. In mast cells, T1 gene transcription is initiated 10.5 kb further upstream than in fibroblasts and gives rise predominantly to the 5-kb transcript under normal growth conditions. Here we demonstrate that calcium ionophore stimulation of mast cells resulted in an upregulation of T1 gene expression and a switch from the long to the short T1 transcript. This was paralleled by the disappearance of the receptor-type T1 protein on the mast cell surface and the secretion of large amounts of the truncated T1 protein. c-Fos and a T1 enhancer, which have previously been identified to be essential for T1 expression in fibroblasts, were not required for calcium ionophore-mediated T1 gene upregulation. Overexpression of the transcription factor GATA-1 in mast cells caused elevated T1 synthesis. Three GATA elements were identified in the minimal GATA-responsive mast cell promoter. Mutational analysis revealed that all three GATA elements are involved in T1 gene expression. Point mutations within the middle GATA element eliminated promoter activity completely, while mutations of the distal and proximal GATA binding sites reduced promoter strength by factors of 2 and 5, respectively. Exogenous expression of GATA-1 was not sufficient to activate the mast cell-specific promoter in NIH 3T3 fibroblasts.

摘要

小鼠延迟早期血清反应基因T1编码白细胞介素-1受体家族的糖蛋白。成纤维细胞中的转录起始受c-Fos调控,并产生一种罕见的5 kb mRNA和一种丰富的2.7 kb mRNA。这些转录本被翻译成一种受体样膜锚定蛋白和一种仅由胞外域组成的分泌蛋白。在肥大细胞中,T1基因转录起始位点比成纤维细胞上游10.5 kb,在正常生长条件下主要产生5 kb转录本。在此我们证明,钙离子载体刺激肥大细胞会导致T1基因表达上调,并从长T1转录本转变为短T1转录本。这伴随着肥大细胞表面受体型T1蛋白的消失以及大量截短型T1蛋白的分泌。c-Fos和一个T1增强子,此前已被确定对成纤维细胞中T1表达至关重要,但钙离子载体介导的T1基因上调并不需要它们。转录因子GATA-1在肥大细胞中的过表达导致T1合成增加。在最小的GATA反应性肥大细胞启动子中鉴定出三个GATA元件。突变分析表明,所有三个GATA元件都参与T1基因表达。中间GATA元件内的点突变完全消除了启动子活性,而远端和近端GATA结合位点的突变分别使启动子强度降低了2倍和5倍。GATA-1的外源表达不足以激活NIH 3T3成纤维细胞中的肥大细胞特异性启动子。

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