Second-Generation Triple Reporter for Bioluminescence, Micro–Positron Emission Tomography, and Fluorescence Imaging

Second-Generation Triple Reporter for Bioluminescence, Micro–Positron Emission Tomography, and Fluorescence Imaging

Bioluminescence, positron emission tomography (PET), and fluorescence modalities are currently available for noninvasive imaging in vivo, each with its own merits. To exploit the combined strengths of each and facilitate multimodality imaging, we engineered a dual-reporter construct in which firefly...

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Veröffentlicht in:Molecular imaging 2006-10, Vol.5 (4), p.465-474
Hauptverfasser: Kesarwala, Aparna H., Prior, Julie L., Sun, Jinwu, Harpstrite, Scott E., Sharma, Vijay, Piwnica-Worms, David
Format: Artikel
Sprache:eng
Schlagworte:
Acyclovir - analogs & derivatives
Acyclovir - pharmacokinetics
Animals
Cell Line
Flow Cytometry - methods
Genes, Reporter
Guanine - analogs & derivatives
Guanine - pharmacokinetics
HeLa Cells
Humans
Luciferases, Firefly - genetics
Luminescence
Luminescent Agents
Mice
Microscopy, Fluorescence - methods
Positron-Emission Tomography - methods
Recombinant Fusion Proteins - genetics
Recombinant Fusion Proteins - pharmacokinetics
Simplexvirus - enzymology
Simplexvirus - genetics
Thymidine Kinase - genetics
Transfection
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Zusammenfassung:Bioluminescence, positron emission tomography (PET), and fluorescence modalities are currently available for noninvasive imaging in vivo, each with its own merits. To exploit the combined strengths of each and facilitate multimodality imaging, we engineered a dual-reporter construct in which firefly luciferase (FLuc) and a 12–amino acid nonstructural linker were fused in frame to the N-terminus of a mutant herpes simplex virus thymidine kinase (mNLS-SR39TK) kinetically enhanced for positron emission tomography (PET). Furthermore, a triple-reporter construct was developed in which monster green fluorescent protein (MGFP), a recently available enhanced fluorescent protein, was introduced into the fusion vector downstream of an internal ribosome entry site (IRES) to allow analysis by fluorescence microscopy or flow cytometry without compromising the specific activities of the upstream fusion components. FLuc bioluminescence was measured with a cooled charge-coupled device camera and mNLS-SR39TK activity by 9-[4-[18F]fluoro-3-(hydroxymethyl) butyl guanine (18F-FHBG) microPET or 3H-penciclovir net accumulation. Importantly, HeLa cells transiently transfected with the FLuc-mNLS-SR39TK-IRES-MGFP triple reporter retained the same specific activities of the FLuc-mNLS-SR39TK heteroenzyme and the individual unfused enzymes with no change in protein half-lives. The presence of the IRES-MGFP modestly decreased upstream heteroprotein expression. In living mice, somatic gene transfer of a ubiquitin promoter-driven FLuc-mNLS-SR39TK-IRES-MGFP plasmid showed a > 1,000-fold increase in liver photon flux and a > 2-fold increase in liver retention of 18F-FHBG by microPET compared with mice treated with control plasmid. Multifocal hepatocellular fluorescence was readily observed by standard confocal microscopy. This second-generation triple reporter incorporating enhanced components enables bioluminescence, PET, and fluorescence imaging of cells and living animals.
ISSN:1535-3508
1536-0121
DOI:10.2310/7290.2006.00024