共 40 条
Accelerated homologous recombination and subsequent genome modification in Drosophila
被引:142
作者:

Baena-Lopez, Luis Alberto
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Natl Inst Med Res, MRC, London NW7 1AA, England Natl Inst Med Res, MRC, London NW7 1AA, England

Alexandre, Cyrille
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Natl Inst Med Res, MRC, London NW7 1AA, England Natl Inst Med Res, MRC, London NW7 1AA, England

Mitchell, Alice
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Natl Inst Med Res, MRC, London NW7 1AA, England Natl Inst Med Res, MRC, London NW7 1AA, England

Pasakarnis, Laurynas
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Natl Inst Med Res, MRC, London NW7 1AA, England Natl Inst Med Res, MRC, London NW7 1AA, England

Vincent, Jean-Paul
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Natl Inst Med Res, MRC, London NW7 1AA, England Natl Inst Med Res, MRC, London NW7 1AA, England
机构:
[1] Natl Inst Med Res, MRC, London NW7 1AA, England
来源:
DEVELOPMENT
|
2013年
/
140卷
/
23期
基金:
欧洲研究理事会;
英国医学研究理事会;
英国惠康基金;
关键词:
Drosophila;
Functional genomics;
Gene targeting;
Homologous recombination;
GUIDED CAS9 NUCLEASE;
HUMAN-CELLS;
ENDS-OUT;
GENE;
EFFICIENT;
SYSTEM;
MELANOGASTER;
TALEN;
TRANSGENESIS;
EXPRESSION;
D O I:
10.1242/dev.100933
中图分类号:
Q [生物科学];
学科分类号:
07 ;
0710 ;
09 ;
摘要:
Gene targeting by 'ends-out' homologous recombination enables the deletion of genomic sequences and concurrent introduction of exogenous DNA with base-pair precision without sequence constraint. In Drosophila, this powerful technique has remained laborious and hence seldom implemented. We describe a targeting vector and protocols that achieve this at high frequency and with very few false positives in Drosophila, either with a two-generation crossing scheme or by direct injection in embryos. The frequency of injection-mediated gene targeting can be further increased with CRISPR-induced double-strand breaks within the region to be deleted, thus making homologous recombination almost as easy as conventional transgenesis. Our targeting vector replaces genomic sequences with a multifunctional fragment comprising an easy-to-select genetic marker, a fluorescent reporter, as well as an attP site, which acts as a landing platform for reintegration vectors. These vectors allow the insertion of a variety of transcription reporters or cDNAs to express tagged or mutant isoforms at endogenous levels. In addition, they pave the way for difficult experiments such as tissue-specific allele switching and functional analysis in post-mitotic or polyploid cells. Therefore, our method retains the advantages of homologous recombination while capitalising on the mutagenic power of CRISPR.
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页码:4818 / +
页数:18
相关论文
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