Literature DB >> 2237639

Targeted gene replacement at the endogenous APRT locus in CHO cells.

G M Adair1, R S Nairn, J H Wilson, J B Scheerer, K A Brotherman.   

Abstract

We demonstrate the feasibility of targeted gene replacement at an endogenous, chromosomal gene locus in cultured mammalian cells, employing a two-step strategy similar to an approach routinely used for genetic manipulation in yeast. Utilizing an APRT+ recombinant generated by targeted integration of plasmid sequences (including a functional copy of the gpt gene) at the CHO APRT locus, we have been able to select gpt- "pop-out" recombinants that have arisen by intrachromosomal recombination between APRT direct repeats at the targeted integration site. Reciprocal exchanges leading to "pop-out" of integrated plasmid/gpt gene sequences occur at a rate of approximately 6.3 x 10(-6) per cell generation. Depending on the site of crossover, such "pop-out" events result in either replacement or restoration of the original APRT target gene sequence.

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Year:  1990        PMID: 2237639     DOI: 10.1007/bf01233193

Source DB:  PubMed          Journal:  Somat Cell Mol Genet        ISSN: 0740-7750


  4 in total

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2.  Gene targeting in Chinese hamster ovary cells is conservative.

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3.  Homology dependence of targeted recombination at the Chinese hamster APRT locus.

Authors:  J B Scheerer; G M Adair
Journal:  Mol Cell Biol       Date:  1994-10       Impact factor: 4.272

4.  A caveat in mouse genetic engineering: ectopic gene targeting in ES cells by bidirectional extension of the homology arms of a gene replacement vector carrying human PARP-1.

Authors:  Aswin Mangerich; Harry Scherthan; Jörg Diefenbach; Ulrich Kloz; Franciscus van der Hoeven; Sascha Beneke; Alexander Bürkle
Journal:  Transgenic Res       Date:  2008-11-26       Impact factor: 2.788

  4 in total

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