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细胞生长状态对丁酸盐处理的HT-29细胞中肠上皮细胞基因表达有不同程度的调节作用。

Cellular growth state differentially regulates enterocyte gene expression in butyrate-treated HT-29 cells.

作者信息

Hodin R A, Meng S, Archer S, Tang R

机构信息

Department of Surgery, Beth Israel Hospital, Harvard Medical School, Boston, MA 02215, USA.

出版信息

Cell Growth Differ. 1996 May;7(5):647-53.

PMID:8732674
Abstract

Enterocyte differentiation occurs at the crypt-villus junction through the transcriptional activation of cell-specific genes, including the brush-border enzyme intestinal alkaline phosphatase (IAP) and the microvillar structural protein, villin. Based upon previous in vivo studies demonstrating that IAP and villin are differentially affected by alterations in epithelial growth state, we examined the regulation of these two genes in an in vitro model of enterocyte differentiation. HT-29 cells were maintained in DMEM + 10% FCS and treated with sodium butyrate to induce enterocyte differentiation. Cell count and [3H]thymidine measurements confirm that sodium butyrate causes a marked decrease in cellular growth state, consistent with the differentiation process. Northern blot analyses revealed time- and dose-dependent increases (P < 0.001) in steady-state IAP and villin mRNA levels. The increases in both IAP and villin expression were dependent upon the presence of one or more newly synthesized proteins. Post-confluence and serum starvation were used to cause cell cycle withdrawal prior to the differentiation process. As predicted from our previous in vivo data, villin expression was unaffected by changes in cellular growth state, whereas IAP expression was dramatically diminished under hypoproliferative conditions. We conclude that early withdrawal from the cell cycle alters the course of enterocyte differentiation, specifically decreasing IAP expression.

摘要

肠上皮细胞分化通过细胞特异性基因的转录激活在隐窝 - 绒毛交界处发生,这些基因包括刷状缘酶肠碱性磷酸酶(IAP)和微绒毛结构蛋白绒毛蛋白。基于先前的体内研究表明IAP和绒毛蛋白受上皮生长状态改变的影响不同,我们在肠上皮细胞分化的体外模型中研究了这两个基因的调控。HT - 29细胞维持在含10%胎牛血清的DMEM中,并用丁酸钠处理以诱导肠上皮细胞分化。细胞计数和[3H]胸苷测量证实丁酸钠导致细胞生长状态显著下降,这与分化过程一致。Northern印迹分析显示稳态IAP和绒毛蛋白mRNA水平呈时间和剂量依赖性增加(P < 0.001)。IAP和绒毛蛋白表达的增加均依赖于一种或多种新合成蛋白质的存在。在分化过程之前,使用汇合后和血清饥饿使细胞退出细胞周期。正如我们先前体内数据所预测的,绒毛蛋白表达不受细胞生长状态变化的影响,而在增殖不足的条件下IAP表达显著降低。我们得出结论,早期退出细胞周期会改变肠上皮细胞分化的进程,特别是降低IAP的表达。

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