Negative Selection with the Diphtheria toxin A fragment Gene Improves Frequency of Cre-Mediated Cassette Exchange in ES Cells

doi:10.1093/jb/mvj208

Journal of Biochemistry Advance Access originally published online on October 15, 2006
Journal of Biochemistry 2006 140(6):793-798; doi:10.1093/jb/mvj208

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Negative Selection with the Diphtheria toxin A fragment Gene Improves Frequency of Cre-Mediated Cassette Exchange in ES Cells

Kimi Araki¹^,*, Masatake Araki² and Ken-ichi Yamamura¹

¹ Department of Developmental Genetics, Institute of Molecular Embryology and Genetics, and ² Institute of Resource Development and Analysis, Kumamoto University, Honjo 2-2-1, Kumamoto 860-0811

^* To whom correspondence should be addressed. E-mail: arakimi{at}gpo.kumamoto-u.ac.jp

Abstract

The Cre-lox system is an important tool for genetic manipulationin embryonic stem cells. We previously reported that the cassetteexchange strategy using the mutant lox66/71 and lox2272 combinationshowed high recombination efficiency and stability. However,the efficiency was strongly affected by the position of chromosomaltarget lox sites. To enrich successful cassette exchange events,even in clones showing lower recombination efficiency, we haveimproved exchange vector. The Diphtheria toxin A fragment genewas placed in the un-exchanged region for negative selectionand the puromycin N-acetyltransferase gene, instead of the neomycinphosphotransferase gene, was used for positive selection. Byreducing random integration, the frequency of successful cassetteexchange increased up to 2–4 fold. Furthermore, by addingthe third lox site to induce intrarmolecular recombination,the recombination efficiency of cassette exchange itself wasimproved, and the frequency increased to maximum 5 fold, inwhich the percentage of exchanged clones reached to 50–70%.This strategy should be useful for other recombinase-mediatedcassette exchanges.

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Negative Selection with the Diphtheria toxin A fragment Gene Improves Frequency of Cre-Mediated Cassette Exchange in ES Cells