Here's another paper (full). Different study - this one is on myelination and tamoxifen. They are also using GM mice, which don't produce FGF. After reading this and a few other studies, I would say this looks interesting enough for clinic trials. It's already used in humans for breast cancer, etc.
http://digitalcommon...arch="tamoxifen fgf"
Edit: tapatalk, big thumbs.
You don't understand. These animals were genetically altered (programmed) to respond to Tamoxifen in a specific way. Tamoxifen is used to trigger the genetically altered program. Humans don't have such a genetic alteration, so Tamoxifen will do nothing like this for humans.
I thought they were programmed not to produce FGF?
Whatever they were programmed to do, it is a program
artificially inserted on purpose in the genetically modified mice to be triggered by tamoxifen, so that they can use tamoxifen to modulate the activity of whatever gene they programmed the mouse to activate/deactivate in response to tamoxifen - the choice of tamoxifen for this is quite arbitrary, since many other substances could have been used as the trigger. Wild type mice (or humans) do not have that artificial program, so tamoxifen will do nothing like that for them (or us).
Here is some more information on the technique:
Dev Biol. 2002 Apr 15;244(2):305-18.
Efficient recombination in diverse tissues by a tamoxifen-inducible form of Cre: a tool for temporally regulated gene activation/inactivation in the mouse.
Hayashi S, McMahon AP.
Source
Department of Molecular and Cellular Biology, Harvard University, 16 Divinity Avenue, Cambridge, Massachusetts 02138, USA.
Abstract
In recent years, the Cre integrase from bacteriophage P1 has become an essential tool for conditional gene activation and/or inactivation in mouse. In an earlier report, we described a fusion protein between Cre and a mutated form of the ligand binding domain of the estrogen receptor (Cre-ER) that renders Cre activity tamoxifen ™ inducible, allowing for conditional modification of gene activity in the mammalian neural tube in utero. In the current work, we have generated a transgenic mouse line in which Cre-ER is ubiquitously expressed to permit temporally regulated Cre-mediated recombination in diverse tissues of the mouse at embryonic and adult stages. We demonstrate that a single, intraperitoneal injection of TM into a pregnant mouse at 8.5 days postcoitum leads to detectable recombination in the developing embryo within 6 h of injection and efficient recombination of a reporter gene in derivatives of all three germ layers within 24 h of injection. In addition, by varying the dose of TM injected, the percentage of cells undergoing a recombination event in the embryo can be controlled. Dose-dependent excision induced by TM was also possible in diverse tissues in the adult mouse, including the central nervous system, and in cultured cells derived from the transgenic mouse line. This inducible Cre system will be a broadly useful tool to modulate gene activity in mouse embryos, adults, and culture systems where temporal control is an important consideration.
Edited by viveutvivas, 01 October 2012 - 08:37 PM.
