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通过位点特异性重组从整合的逆转录病毒载体中切除特定DNA序列。

Excision of specific DNA-sequences from integrated retroviral vectors via site-specific recombination.

作者信息

Bergemann J, Kühlcke K, Fehse B, Ratz I, Ostertag W, Lother H

机构信息

Heinrich-Pette-Institut für Experimentelle Virologie und Immunologie, Universität Hamburg, Germany.

出版信息

Nucleic Acids Res. 1995 Nov 11;23(21):4451-6. doi: 10.1093/nar/23.21.4451.

Abstract

Vectors for gene transfer and gene therapy were developed which combine the advantages of the integrase and recombinase systems. This was achieved by inserting two loxP sites for specific DNA excision into an MESV based retroviral vector. We show that this 'retroviral lox system' allows the infection of cells and the expression of transferred genes. In addition, we constructed an efficient retrovirus-based expression system for a modified Cre recombinase. Functional tests for DNA excision from integrated retroviral lox vectors were performed by the use of a negative selectable marker gene (thymidine kinase). Cre expression in cells infected with retroviral lox vectors and subsequent BrdU selection for cells in which site-specific recombination has occurred results in large numbers of independent cell clones. These results were confirmed by detailed molecular analysis. In addition we developed retroviral suicide vectors in which the enhancer/promoter elements of both LTRs were replaced by lox sequences. We show that lox-sequences located in the LTRs of retroviral vectors are stable during retroviral replication. Potential applications of this system would be the establishment of revertants of retrovirus-infected cells by controlled excision of nearly the complete proviral DNA.

摘要

开发了用于基因转移和基因治疗的载体,其结合了整合酶和重组酶系统的优点。这是通过将两个用于特异性DNA切除的loxP位点插入基于MESV的逆转录病毒载体中来实现的。我们表明,这种“逆转录病毒lox系统”允许细胞感染和转移基因的表达。此外,我们构建了一种用于修饰的Cre重组酶的高效逆转录病毒表达系统。通过使用阴性选择标记基因(胸苷激酶)对整合的逆转录病毒lox载体进行DNA切除的功能测试。在感染逆转录病毒lox载体的细胞中表达Cre,并随后对发生位点特异性重组的细胞进行BrdU选择,可产生大量独立的细胞克隆。详细的分子分析证实了这些结果。此外,我们开发了逆转录病毒自杀载体,其中两个LTR的增强子/启动子元件被lox序列取代。我们表明,位于逆转录病毒载体LTR中的lox序列在逆转录病毒复制过程中是稳定的。该系统的潜在应用将是通过几乎完全切除前病毒DNA的受控切除来建立逆转录病毒感染细胞的回复体。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/e437/307403/3f8bb4eca1f2/nar00021-0235-a.jpg

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