共 18 条
Unmodified Cre recombinase crosses the membrane
被引:48
作者:

Will, E
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机构: Heinrich Pette Inst Expt Virol & Immunol, Dept Cell & Virus Genet, D-20251 Hamburg, Germany

Klump, H
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机构: Heinrich Pette Inst Expt Virol & Immunol, Dept Cell & Virus Genet, D-20251 Hamburg, Germany

Heffner, N
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h-index: 0
机构: Heinrich Pette Inst Expt Virol & Immunol, Dept Cell & Virus Genet, D-20251 Hamburg, Germany

Schwieger, M
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机构: Heinrich Pette Inst Expt Virol & Immunol, Dept Cell & Virus Genet, D-20251 Hamburg, Germany

Schiedlmeier, B
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机构: Heinrich Pette Inst Expt Virol & Immunol, Dept Cell & Virus Genet, D-20251 Hamburg, Germany

Ostertag, W
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机构: Heinrich Pette Inst Expt Virol & Immunol, Dept Cell & Virus Genet, D-20251 Hamburg, Germany

Baum, C
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机构: Heinrich Pette Inst Expt Virol & Immunol, Dept Cell & Virus Genet, D-20251 Hamburg, Germany

Stocking, C
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机构: Heinrich Pette Inst Expt Virol & Immunol, Dept Cell & Virus Genet, D-20251 Hamburg, Germany
机构:
[1] Heinrich Pette Inst Expt Virol & Immunol, Dept Cell & Virus Genet, D-20251 Hamburg, Germany
[2] Hannover Med Sch, Dept Hematol & Oncol, D-30625 Hannover, Germany
关键词:
D O I:
10.1093/nar/gnf059
中图分类号:
Q5 [生物化学];
Q7 [分子生物学];
学科分类号:
071010 ;
081704 ;
摘要:
Site-specific recombination in genetically modified cells can be achieved by the activity of Cre recombinase from bacteriophage P1. Commonly an expression vector encoding Cre Is introduced into cells; however, this can lead to undesired side-effects. Therefore, we tested whether cell-permeable Cre fusion proteins can be directly used for lox-specific recombination in a cell line tailored to shift from red to green fluorescence after loxP-specific recombination. Comparison of purified recombinant Cre proteins with and without a heterologous 'protein transduction domain' surprisingly showed that the unmodified Cre recombinase already possesses an intrinsic ability to cross the membrane border. Addition of purified recombinant Cre enyzme to primary bone marrow cells Isolated from transgenic C/EBPalpha(fl/fl) mice also led to excision of the 'floxed' C/EBPalpha gene, thus demonstrating its potential for in vivo applications. We conclude that Cre enyzme itself or its intrinsic membrane-permeating moiety are attractive tools for direct manipulation of mammalian cells.
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