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哺乳动物基因组的靶向修饰。

Targeted modification of mammalian genomes.

作者信息

Sorrell David A, Kolb Andreas F

机构信息

Molecular Recognition Group, Hannah Research Institute, Ayr, KA6 5HL, UK.

出版信息

Biotechnol Adv. 2005 Nov;23(7-8):431-69. doi: 10.1016/j.biotechadv.2005.03.003.

DOI:10.1016/j.biotechadv.2005.03.003
PMID:15925473
Abstract

The stable and site-specific modification of mammalian genomes has a variety of applications in biomedicine and biotechnology. Here we outline two alternative approaches that can be employed to achieve this goal: homologous recombination (HR) or site-specific recombination. Homologous recombination relies on sequence similarity (or rather identity) of a piece of DNA that is introduced into a host cell and the host genome. In most cell types, the frequency of homologous recombination is markedly lower than the frequency of random integration. Especially in somatic cells, homologous recombination is an extremely rare event. However, recent strategies involving the introduction of DNA double-strand breaks, triplex forming oligonucleotides or adeno-associated virus can increase the frequency of homologous recombination. Site-specific recombination makes use of enzymes (recombinases, transposases, integrases), which catalyse DNA strand exchange between DNA molecules that have only limited sequence homology. The recognition sites of site-specific recombinases (e.g. Cre, Flp or PhiC31 integrase) are usually 30-50 bp. In contrast, retroviral integrases only require a specific dinucleotide sequence to insert the viral cDNA into the host genome. Depending on the individual enzyme, there are either innumerable or very few potential target sites for a particular integrase/recombinase in a mammalian genome. A number of strategies have been utilised successfully to alter the site-specificity of recombinases. Therefore, site-specific recombinases provide an attractive tool for the targeted modification of mammalian genomes.

摘要

哺乳动物基因组的稳定且位点特异性修饰在生物医学和生物技术领域有多种应用。在此,我们概述两种可用于实现这一目标的替代方法:同源重组(HR)或位点特异性重组。同源重组依赖于导入宿主细胞的一段DNA与宿主基因组之间的序列相似性(确切地说是同一性)。在大多数细胞类型中,同源重组的频率明显低于随机整合的频率。尤其是在体细胞中,同源重组是极其罕见的事件。然而,最近涉及引入DNA双链断裂、三链形成寡核苷酸或腺相关病毒的策略可以提高同源重组的频率。位点特异性重组利用酶(重组酶、转座酶、整合酶),这些酶催化仅具有有限序列同源性的DNA分子之间的DNA链交换。位点特异性重组酶(如Cre、Flp或PhiC31整合酶)的识别位点通常为30 - 50个碱基对。相比之下,逆转录病毒整合酶仅需要特定的二核苷酸序列就能将病毒cDNA插入宿主基因组。根据具体的酶,在哺乳动物基因组中,特定整合酶/重组酶的潜在靶位点要么有无数个,要么非常少。已经成功利用了许多策略来改变重组酶的位点特异性。因此,位点特异性重组酶为哺乳动物基因组的靶向修饰提供了一种有吸引力的工具。

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