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人肠道上皮细胞中志贺样毒素1受体——球三糖神经酰胺的成熟调控

Maturational regulation of globotriaosylceramide, the Shiga-like toxin 1 receptor, in cultured human gut epithelial cells.

作者信息

Jacewicz M S, Acheson D W, Mobassaleh M, Donohue-Rolfe A, Balasubramanian K A, Keusch G T

机构信息

Division of Geographic Medicine and Infectious Diseases, Tupper Research Institute, New England Medical Center, Boston, Massachusetts 02111, USA.

出版信息

J Clin Invest. 1995 Sep;96(3):1328-35. doi: 10.1172/JCI118168.

DOI:10.1172/JCI118168
PMID:7657808
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC185755/
Abstract

Differentiated villus intestinal epithelial cells express globotriaosylceramide, the Shiga-like toxin 1 (SLT-1) receptor, and are sensitive to toxin-mediated cytotoxicity, whereas undifferentiated crypt cells neither express Gb3 nor respond to toxin. To investigate if SLT-1 receptors are maturationally regulated in human intestinal cells, we examined the effect of butyrate, a known transcriptional regulator of differentiation genes in many cell types, using cultured colonic cancer-derived epithelial cell lines. Exposure to butyrate increased villus cell marker enzymes such as alkaline phosphatase, sucrase, and lactase, expression of toxin receptors, and sensitivity to SLT-1 in villus-like CaCo-2A and HT-29 cells. These effects were reversibly inhibited by preincubation of CaCo-2A cells with actinomycin D or cycloheximide. Butyrate-treated CaCo-2A cells unable to bind fluoresceinated SLT-1 B subunit were undifferentiated as assessed by alkaline phosphatase activity. HT-29 cells induced to differentiate by another signal, glucose deprivation, upregulated receptor content and response to toxin. Crypt-like T-84 cells responded to butyrate with a modest increase in alkaline phosphatase and toxin binding, but no induction of sucrase or lactase, and no change in sensitivity to toxin. The results demonstrate that expression of SLT-1 toxin receptors and toxin sensitivity are coregulated with cellular differentiation in cultured intestinal cells.

摘要

分化的绒毛肠上皮细胞表达球三糖神经酰胺,即志贺样毒素1(SLT-1)受体,并且对毒素介导的细胞毒性敏感,而未分化的隐窝细胞既不表达Gb3也不响应毒素。为了研究SLT-1受体在人肠道细胞中是否受成熟调控,我们使用培养的结肠癌来源的上皮细胞系,检测了丁酸盐(一种已知的多种细胞类型中分化基因的转录调节因子)的作用。暴露于丁酸盐可增加绒毛状CaCo-2A和HT-29细胞中绒毛细胞标记酶如碱性磷酸酶、蔗糖酶和乳糖酶的表达、毒素受体的表达以及对SLT-1的敏感性。用放线菌素D或环己酰亚胺预孵育CaCo-2A细胞可可逆地抑制这些作用。通过碱性磷酸酶活性评估,不能结合荧光素化SLT-1 B亚基的丁酸盐处理的CaCo-2A细胞未分化。通过另一种信号即葡萄糖剥夺诱导分化的HT-29细胞,其受体含量上调且对毒素的反应增强。隐窝样T-84细胞对丁酸盐的反应是碱性磷酸酶和毒素结合适度增加,但蔗糖酶或乳糖酶未诱导表达,对毒素的敏感性也无变化。结果表明,在培养的肠道细胞中,SLT-1毒素受体的表达和毒素敏感性与细胞分化共同受到调节。

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