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源自增强子捕获逆转录病毒的整合前病毒的高频表达。

High frequency expression of integrated proviruses derived from enhancer trap retroviruses.

作者信息

Sablitzky F, Jönsson J I, Cohen B L, Phillips R A

机构信息

Department of Molecular and Medical Genetics, University of Toronto, Ontario, Canada.

出版信息

Cell Growth Differ. 1993 Jun;4(6):451-9.

PMID:8373730
Abstract

Since retroviruses integrate preferentially into transcriptionally active loci, the provirus may come under the control of regulatory elements of the gene into which it integrated and thus become a functional tag for that gene. In order to determine the frequency of retroviral integration near active endogenous enhancer elements, a retroviral enhancer trap vector was constructed. Lacking the long terminal repeat enhancer, expression of the neomycin resistance (neo) gene, used as a reporter, is dependent upon endogenous enhancer elements able to activate the long terminal repeat promoter. Infection of murine fibroblast cells indicated that a high proportion of the proviral copies expressed the neo gene. Infection of hematopoietic lines confirmed this high frequency of expression of integrated proviruses. Overall, between 43 and 74% of proviruses integrated into several different cell lines expressed the neo gene. These data suggest that retroviral integration is not only dependent upon transcriptional activity of the genomic target sites, but, more specifically, retroviruses preferentially integrate near active enhancer elements which are often associated with developmentally regulated genes.

摘要

由于逆转录病毒优先整合到转录活跃位点,前病毒可能受其整合位点基因的调控元件控制,从而成为该基因的功能性标签。为了确定逆转录病毒在活跃的内源性增强子元件附近的整合频率,构建了一种逆转录病毒增强子捕获载体。由于缺乏长末端重复序列增强子,用作报告基因的新霉素抗性(neo)基因的表达依赖于能够激活长末端重复序列启动子的内源性增强子元件。对鼠成纤维细胞的感染表明,很大比例的前病毒拷贝表达了neo基因。对造血系的感染证实了整合的前病毒的高表达频率。总体而言,整合到几种不同细胞系中的前病毒中有43%至74%表达了neo基因。这些数据表明,逆转录病毒整合不仅依赖于基因组靶位点的转录活性,更具体地说,逆转录病毒优先整合到活跃的增强子元件附近,这些元件通常与发育调控基因相关。

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