2001
DOI: 10.1101/gad.892001
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The lac operator-repressor system is functional in the mouse

Abstract: We report the successful transfer of a fully functional lac operator-repressor gene regulatory system to the mouse. The key component is a lac repressor transgene that resembles a typical mammalian gene both in codon usage and structure and expresses functional levels of repressor protein in the animal. We used the repressor to regulate the expression of a mammalian reporter gene consisting of the tyrosinase promoter embedded with three short lac operator sequences and the tyrosinase coding sequence. Pigmentat… Show more

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Cited by 144 publications
(157 citation statements)
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“…For in vivo induction, 10 mM IPTG was added to mouse drinking water 3 days after i.p. infection (45), and spleens were harvested 24 -48 h later. Low density splenocytes were isolated by brief incubation with collagenase, followed by separation in dense BSA gradient (42), and used as APC as described.…”
Section: Induction Of Intracellular Flic Expressionmentioning
confidence: 99%
“…For in vivo induction, 10 mM IPTG was added to mouse drinking water 3 days after i.p. infection (45), and spleens were harvested 24 -48 h later. Low density splenocytes were isolated by brief incubation with collagenase, followed by separation in dense BSA gradient (42), and used as APC as described.…”
Section: Induction Of Intracellular Flic Expressionmentioning
confidence: 99%
“…One way of circumventing this problem is to utilize an inducible system regulating the expression of the transgene. Here we modified the inducible SV40 / humanized LacI system previously developed for transgenic mouse models [3]. The system has advantages for this application such as low background expression, high inducibility above background and an inexpensive inducing agent that is amenable to both in vitro and in vivo use.…”
Section: Discussionmentioning
confidence: 99%
“…Recombinant DNA techniques PTEN Inducible system-Humanized LacI and the inducible SV40 promoter have been described elsewhere [3]. The LacI cDNA was cloned into pIRESpuro2 (Clonetech, Mountain View, CA, USA) at the Eco RI site.…”
Section: Methodsmentioning
confidence: 99%
“…Accordingly, many approaches such as knockdown with synthesized morpholinos, insertional mutagenesis, ectopic expression of a target gene, dominantnegative and conditional gene expression, have been developed to elucidate gene functions during embryonic development. Several inducible gene expression systems including the ecdysone-regulated gene switch (Triezenberg et al, 1988), the lac operator-repressor system (Cronin et al, 2001), the inducible GAL4/UAS system (Lycett et al, 2004) and two tetracycline (Tet)-controlled systems (Gossen and Bujard, 1992;Gossen et al, 1995) have been developed for manipulating gene expression at the transcriptional level in Drosophila, mammalian cells and transgenic animals with varying degrees of success, but their activities in zebrafish are not yet well-characterized. In fact, only a limited number of transgenic zebrafish lines carrying these gene expression systems are currently available.…”
Section: Introductionmentioning
confidence: 99%