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基于功能表征克隆变异和组织特异性基因调控因子的体内系统。

In vivo system for characterizing clonal variation and tissue-specific gene regulatory factors based on function.

作者信息

Hardeman E C, Minty A, Benton-Vosman P, Kedes L, Blau H M

机构信息

Department of Pharmacology, Stanford University School of Medicine, California 94305-5332.

出版信息

J Cell Biol. 1988 Apr;106(4):1027-34. doi: 10.1083/jcb.106.4.1027.

Abstract

The inducibility of stably transfected alpha-cardiac actin genes differs among L cell clones. We examined the ability of muscle-specific factors to induce the expression of the human muscle alpha-cardiac actin gene promoter when stably transfected into mouse fibroblast L cells. This promoter is transcriptionally active in L cells at a low level, 2-5% of that in transfected muscle cells. Upon fusion with muscle cells to form heterokaryons, expression of the transfected alpha-cardiac actin gene promoter can be induced. However, induction is observed with only 10% of transfected L cell clones and the magnitude of this induction varies between 5- and 50-fold. These properties of the transfected L cell appear to be stably inherited. Our results are consistent with the hypothesis that muscle cells contain factors capable of increasing the transcription of the transfected gene, but that differences among L cell clones, possibly in the site of integration in the genome, determine the extent to which the gene can respond. By fusion into heterokaryons, transfectants with responsive genes can be identified. Such clones should prove useful in determining the basis for clonal variation. In addition, they provide an in vivo system for isolating functionally active tissue-specific transcription factors and the genes that encode them.

摘要

稳定转染的α-心肌肌动蛋白基因的诱导性在L细胞克隆之间存在差异。我们检测了肌肉特异性因子在稳定转染入小鼠成纤维细胞L细胞后诱导人肌肉α-心肌肌动蛋白基因启动子表达的能力。该启动子在L细胞中的转录活性较低,仅为转染肌肉细胞中的2%-5%。与肌肉细胞融合形成异核体后,转染的α-心肌肌动蛋白基因启动子的表达可被诱导。然而,只有10%的转染L细胞克隆能观察到诱导现象,且诱导程度在5到50倍之间变化。转染L细胞的这些特性似乎能稳定遗传。我们的结果与以下假设一致:肌肉细胞含有能够增加转染基因转录的因子,但L细胞克隆之间的差异,可能在于基因组中的整合位点,决定了基因的响应程度。通过融合形成异核体,可以鉴定出具有响应基因的转染子。这样的克隆在确定克隆变异的基础方面应是有用的。此外,它们为分离功能活性组织特异性转录因子及其编码基因提供了一个体内系统。

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