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条件永生化肠上皮细胞:研究分化肠细胞的新方法。

Conditionally immortalized intestinal epithelial cells: novel approach for study of differentiated enterocytes.

作者信息

Paul E C, Hochman J, Quaroni A

机构信息

Department of Physiology, Cornell University, Ithaca, New York 14853.

出版信息

Am J Physiol. 1993 Jul;265(1 Pt 1):C266-78. doi: 10.1152/ajpcell.1993.265.1.C266.

DOI:10.1152/ajpcell.1993.265.1.C266
PMID:8393282
Abstract

Clonal cell lines have been established from primary fetal rat intestinal epithelial cells by stable transfection with plasmids containing either the simian virus 40 (SV40) large T-antigen gene under the control of the heavy metal inducible metallothionein promoter (pMTWt) or the thermolabile SV40 T-antigen gene under the control of the SV40 early promoter (pZipSVtsa58). pMTWt-transfected cells produced sufficient T-antigen to allow them to proliferate both when the metallothionein promoter was induced and uninduced. No differences were observed in the pattern of intestinal epithelial markers expressed when the cells were cultured in the presence or absence of inducing agent (zinc). In contrast, fetal rat intestinal epithelial cells transfected with pZipSVtsa58 were immortalized conditionally; cells proliferated at 32 degrees C but ceased to proliferate between 48 and 72 h of culture at 39 degrees C. Four of these cell lines were characterized in detail; they showed microvilli and tight junctions as well as dome formation and expressed functional and biochemical markers of intestinal epithelial cells, including keratins 8, 19, and 21, aminopeptidase N, and dipeptidyl peptidase IV. One cell line, 2/4/A1, expressed in addition a low level of lactase and sucrase-isomaltase. The amount and/or activity of some of these markers changed during the switch from the proliferative to the nonproliferative state (switch from culture at 32 to 39 degrees C), resulting in a more differentiated phenotype and mimicking similar changes taking place during intestinal epithelial cell differentiation in vivo.

摘要

通过用含有在重金属诱导型金属硫蛋白启动子(pMTWt)控制下的猿猴病毒40(SV40)大T抗原基因或在SV40早期启动子(pZipSVtsa58)控制下的温度敏感型SV40 T抗原基因的质粒进行稳定转染,已从原代胎鼠肠上皮细胞建立了克隆细胞系。用pMTWt转染的细胞产生了足够的T抗原,使得它们在金属硫蛋白启动子被诱导和未被诱导时都能增殖。当细胞在有无诱导剂(锌)的情况下培养时,所表达的肠上皮标志物模式未观察到差异。相比之下,用pZipSVtsa58转染的胎鼠肠上皮细胞是条件永生的;细胞在32℃时增殖,但在39℃培养48至72小时之间停止增殖。对其中四个细胞系进行了详细表征;它们显示出微绒毛和紧密连接以及穹窿形成,并表达了肠上皮细胞的功能和生化标志物,包括角蛋白8、19和21、氨肽酶N和二肽基肽酶IV。一个细胞系2/4/A1还额外表达了低水平的乳糖酶和蔗糖酶-异麦芽糖酶。其中一些标志物的量和/或活性在从增殖状态转变为非增殖状态(从32℃培养转变为39℃培养)的过程中发生了变化,导致表型更加分化,模拟了体内肠上皮细胞分化过程中发生的类似变化。

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