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      Tetrazine-Based Cycloadditions: Application to Pretargeted Live Cell Imaging

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          Abstract

          Bioorthogonal tetrazine cycloadditions have been applied to live cell labeling. Tetrazines react irreversibly with the strained dienophile norbornene forming dihydropyrazine products and dinitrogen. The reaction is high yielding, selective, and fast in aqueous media. Her2/neu receptors on live human breast cancer cells were targeted with a monoclonal antibody modified with a norbornene. Tetrazines conjugated to a near-infrared fluorochrome selectively and rapidly label the pretargeted antibody in the presence of serum. These findings indicate that this chemistry is suitable for in vitro labeling experiments, and suggests that it may prove a useful strategy for in vivo pretargeted imaging under numerous modalities.

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          Most cited references23

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          A stepwise huisgen cycloaddition process: copper(I)-catalyzed regioselective "ligation" of azides and terminal alkynes.

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            Tetrazine ligation: fast bioconjugation based on inverse-electron-demand Diels-Alder reactivity.

            Described is a bioorthogonal reaction that proceeds with unusually fast reaction rates without need for catalysis: the cycloaddition of s-tetrazine and trans-cyclooctene derivatives. The reactions tolerate a broad range of functionality and proceed in high yield in organic solvents, water, cell media, or cell lysate. The rate of the ligation between trans-cyclooctene and 3,6-di-(2-pyridyl)-s-tetrazine is very rapid (k2 2000 M-1 s-1). This fast reactivity enables protein modification at low concentration.
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              In vivo imaging of membrane-associated glycans in developing zebrafish.

              Glycans are attractive targets for molecular imaging but have been inaccessible because of their incompatibility with genetically encoded reporters. We demonstrated the noninvasive imaging of glycans in live developing zebrafish, using a chemical reporter strategy. Zebrafish embryos were treated with an unnatural sugar to metabolically label their cell-surface glycans with azides. Subsequently, the embryos were reacted with fluorophore conjugates by means of copper-free click chemistry, enabling the visualization of glycans in vivo at subcellular resolution during development. At 60 hours after fertilization, we observed an increase in de novo glycan biosynthesis in the jaw region, pectoral fins, and olfactory organs. Using a multicolor detection strategy, we performed a spatiotemporal analysis of glycan expression and trafficking and identified patterns that would be undetectable with conventional molecular imaging approaches.
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                Author and article information

                Journal
                Bioconjugate Chemistry
                Bioconjugate Chem.
                American Chemical Society (ACS)
                1043-1802
                1520-4812
                December 17 2008
                November 21 2008
                December 17 2008
                : 19
                : 12
                : 2297-2299
                Affiliations
                [1 ]Center for Molecular Imaging Research, Massachusetts General Hospital/Harvard Medical School Charlestown, Massachusetts 02129, and Center for Systems Biology, Massachusetts General Hospital/Harvard Medical School Boston, Massachusetts 02114
                Article
                10.1021/bc8004446
                2677645
                19053305
                3ba2bc31-0cac-49d0-8179-bd6798e0e372
                © 2008
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