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大鼠肠三叶因子基因的分子克隆。一种与肠杯状细胞相关的启动子的特性。

Molecular cloning of the rat intestinal trefoil factor gene. Characterization of an intestinal goblet cell-associated promoter.

作者信息

Sands B E, Ogata H, Lynch-Devaney K, deBeaumont M, Ezzell R M, Podolsky D K

机构信息

Gastrointestinal Unit, Massachusetts General Hospital, Boston 02114, USA.

出版信息

J Biol Chem. 1995 Apr 21;270(16):9353-61. doi: 10.1074/jbc.270.16.9353.

DOI:10.1074/jbc.270.16.9353
PMID:7721858
Abstract

Intestinal trefoil factor (ITF) is a small peptide bearing the unique motif of intrachain disulfide bonds characteristic of the trefoil family. Previous work had localized expression of ITF primarily within goblet cells in the small and large bowel, making it a candidate gene for the study of the molecular basis of intestinal and goblet cell-specific gene expression. In order to study the regulation of ITF expression, we have cloned the rat ITF gene and sequenced 1.7 kilobases of the 5'-flanking region. RNase protection analysis demonstrated a single transcriptional start site. Various lengths of the 5'-flanking region were linked to the reporter gene luciferase and transfected into the colon cancer cell lines LS174T and Caco-2, representing, respectively, cells with and without goblet cell-like phenotype. Expression in the goblet cell-like LS174T colon cancer cell line was nearly 10-fold greater than expression in Caco-2 cells which exhibit columnar enterocyte-like phenotype. The pattern of goblet cell-associated selective transcription required only 153 base pairs of the rat ITF 5'-flanking sequence. Transfection of a construct of human growth hormone under the control of the rat ITF promoter in the N2 subclone of HT-29 cells demonstrated expression of the reporter gene only in those cells exhibiting a goblet cell phenotype as assessed by expression of immunoreactive mucin. These initial studies of the 5'-flanking region of the ITF gene demonstrate the presence of cis-regulatory elements capable of directing goblet cell specific expression.

摘要

肠三叶因子(ITF)是一种小肽,具有三叶因子家族特有的链内二硫键独特基序。先前的研究已将ITF的表达主要定位在小肠和大肠的杯状细胞内,这使其成为研究肠道和杯状细胞特异性基因表达分子基础的候选基因。为了研究ITF表达的调控,我们克隆了大鼠ITF基因并对其5'侧翼区域的1.7千碱基进行了测序。核糖核酸酶保护分析显示有一个单一的转录起始位点。将不同长度的5'侧翼区域与报告基因荧光素酶连接,并转染到结肠癌细胞系LS174T和Caco-2中,这两种细胞系分别代表具有和不具有杯状细胞样表型的细胞。在具有杯状细胞样的LS174T结肠癌细胞系中的表达比表现为柱状肠上皮细胞样表型的Caco-2细胞中的表达高近10倍。杯状细胞相关的选择性转录模式仅需要大鼠ITF 5'侧翼序列的153个碱基对。在HT-29细胞的N2亚克隆中,在大鼠ITF启动子控制下转染人生长激素构建体,结果显示报告基因仅在那些通过免疫反应性粘蛋白表达评估表现出杯状细胞表型的细胞中表达。这些对ITF基因5'侧翼区域的初步研究表明存在能够指导杯状细胞特异性表达的顺式调控元件。

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J Biol Chem. 1995 Apr 21;270(16):9353-61. doi: 10.1074/jbc.270.16.9353.
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