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多种丝氨酸噬菌体整合酶介导哺乳动物细胞中的位点特异性重组。

A diversity of serine phage integrases mediate site-specific recombination in mammalian cells.

作者信息

Keravala Annahita, Groth Amy C, Jarrahian Sohail, Thyagarajan Bhaskar, Hoyt Jason J, Kirby Patrick J, Calos Michele P

机构信息

Department of Genetics, M-334, Stanford University School of Medicine, 300 Pasteur Drive, Stanford, CA 94305-5120, USA.

出版信息

Mol Genet Genomics. 2006 Aug;276(2):135-46. doi: 10.1007/s00438-006-0129-5. Epub 2006 May 13.

DOI:10.1007/s00438-006-0129-5
PMID:16699779
Abstract

This study evaluated the ability of five serine phage integrases, from phages A118, U153, Bxb1, phiFC1, and phiRV1, to mediate recombination in mammalian cells. Two types of recombination were investigated, including the ability of an integrase to mediate recombination between its own phage att sites in the context of a mammalian cell and the ability of an integrase to perform genomic integration pairing a phage att site with an endogenous mammalian sequence. We demonstrated that the A118 integrase mediated precise intra-molecular recombination of a plasmid containing its attB and attP sites at a frequency of approximately 50% in human cells. The closely related U153 integrase also performed efficient recombination in human cells on a plasmid containing the attB and attP sites of A118. The integrases from phages Bxb1, phiFC1, and phiRV1 carried out such recombination at their attB and attP sites at frequencies ranging from 11 to 75%. Furthermore, the A118 integrase mediated recombination between its attP site on a plasmid and pseudo attB sites in the human genome, i.e. native sequences with partial identity to attB. Fifteen such A118 pseudo att sites were analyzed, and a consensus recognition site was identified. The other integrases did not mediate integration at genomic sequences at a frequency above background. These site-specific integrases represent valuable new tools for manipulating eukaryotic genomes.

摘要

本研究评估了来自噬菌体A118、U153、Bxb1、phiFC1和phiRV1的五种丝氨酸噬菌体整合酶在哺乳动物细胞中介导重组的能力。研究了两种类型的重组,包括整合酶在哺乳动物细胞环境中介导其自身噬菌体附着位点之间重组的能力,以及整合酶将噬菌体附着位点与内源性哺乳动物序列配对进行基因组整合的能力。我们证明,A118整合酶在人细胞中以约50%的频率介导了含有其附着B和附着P位点的质粒的精确分子内重组。密切相关的U153整合酶在含有A118附着B和附着P位点的质粒上也能在人细胞中高效重组。来自噬菌体Bxb1、phiFC1和phiRV1的整合酶在其附着B和附着P位点进行这种重组的频率在11%至75%之间。此外,A118整合酶介导了质粒上的附着P位点与人类基因组中的假附着B位点之间的重组,即与附着B具有部分同一性的天然序列。分析了15个这样的A118假附着位点,并确定了一个共有识别位点。其他整合酶在基因组序列上介导整合的频率未高于背景频率。这些位点特异性整合酶是操纵真核基因组的有价值的新工具。

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Transgenic Xenopus laevis embryos can be generated using phiC31 integrase.
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