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DNA在植物基因组中野生型和突变型lox位点的位点特异性整合。

Site-specific integration of DNA into wild-type and mutant lox sites placed in the plant genome.

作者信息

Albert H, Dale E C, Lee E, Ow D W

机构信息

Plant Gene Expression Center, USDA/ARS-UC Berkeley, Albany 94710, USA.

出版信息

Plant J. 1995 Apr;7(4):649-59. doi: 10.1046/j.1365-313x.1995.7040649.x.

Abstract

The bacteriophage P1 Cre-lox site-specific recombination system has been used to integrate DNA specifically at lox sites previously placed in the tobacco genome. As integrated molecules flanked by wild-type lox sites can readily excise in the presence of Cre recombinase, screening for mutant lox sites that can resist excisional recombination was performed. In gene integration experiments, wild-type and mutant lox sites were used in conjunction with two strategies for abolishing post-integration Cre activity: (i) promoter displacement of a cre-expression construct present in the target genome; and (ii) transient expression of cre. When the promoter displacement strategy was used, integrant plants were recovered after transformation with constructs containing mutant lox sequences, but not with constructs containing wild-type lox sites. When cre was transiently expressed, integrant plants were obtained after transformation with either mutant or wild-type lox sites. DNA rearrangements at the target locus were less frequent when mutant lox sites were used. DNA integration at the genomic lox site was usually without additional insertions in the genome. Thus, the Cre-lox site-specific recombination system is useful for the single-copy integration of DNA into a chromosomal lox site.

摘要

噬菌体P1 Cre-lox位点特异性重组系统已被用于将DNA特异性整合到先前置于烟草基因组中的lox位点。由于在野生型lox位点两侧的整合分子在Cre重组酶存在时可轻易切除,因此对能抵抗切除重组的突变lox位点进行了筛选。在基因整合实验中,野生型和突变型lox位点与两种消除整合后Cre活性的策略一起使用:(i) 置换靶基因组中存在的cre表达构建体的启动子;(ii) cre的瞬时表达。当使用启动子置换策略时,用含有突变lox序列的构建体转化后可获得整合植株,但用含有野生型lox位点的构建体转化则不能。当cre瞬时表达时,用突变型或野生型lox位点转化后均可获得整合植株。使用突变型lox位点时,靶位点处的DNA重排频率较低。基因组lox位点处的DNA整合通常不会在基因组中产生额外插入。因此,Cre-lox位点特异性重组系统可用于将DNA单拷贝整合到染色体lox位点。

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