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Switching on the lights for gene therapy
Authors:Winkeler Alexandra  Sena-Esteves Miguel  Paulis Leonie E M  Li Hongfeng  Waerzeggers Yannic  Rückriem Benedikt  Himmelreich Uwe  Klein Markus  Monfared Parisa  Rueger Maria A  Heneka Michael  Vollmar Stefan  Hoehn Mathias  Fraefel Cornel  Graf Rudolf  Wienhard Klaus  Heiss Wolf D  Jacobs Andreas H
Institution:Laboratory for Gene Therapy and Molecular Imaging at the Max Planck-Institute for Neurological Research, Center for Molecular Medicine (CMMC) and Department of Neurology, University of Cologne, Cologne, Germany.
Abstract:Strategies for non-invasive and quantitative imaging of gene expression in vivo have been developed over the past decade. Non-invasive assessment of the dynamics of gene regulation is of interest for the detection of endogenous disease-specific biological alterations (e.g., signal transduction) and for monitoring the induction and regulation of therapeutic genes (e.g., gene therapy). To demonstrate that non-invasive imaging of regulated expression of any type of gene after in vivo transduction by versatile vectors is feasible, we generated regulatable herpes simplex virus type 1 (HSV-1) amplicon vectors carrying hormone (mifepristone) or antibiotic (tetracycline) regulated promoters driving the proportional co-expression of two marker genes. Regulated gene expression was monitored by fluorescence microscopy in culture and by positron emission tomography (PET) or bioluminescence (BLI) in vivo. The induction levels evaluated in glioma models varied depending on the dose of inductor. With fluorescence microscopy and BLI being the tools for assessing gene expression in culture and animal models, and with PET being the technology for possible application in humans, the generated vectors may serve to non-invasively monitor the dynamics of any gene of interest which is proportionally co-expressed with the respective imaging marker gene in research applications aiming towards translation into clinical application.
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