Literature DB >> 24134212

Simultaneous dual protein labeling using a triorthogonal reagent.

Mohammad Rashidian1, Sidath C Kumarapperuma, Kari Gabrielse, Adrian Fegan, Carston R Wagner, Mark D Distefano.   

Abstract

Construction of heterofunctional proteins is a rapidly emerging area of biotherapeutics. Combining a protein with other moieties, such as a targeting element, a toxic protein or small molecule, and a fluorophore or polyethylene glycol (PEG) group, can improve the specificity, functionality, potency, and pharmacokinetic profile of a protein. Protein farnesyl transferase (PFTase) is able to site-specifically and quantitatively prenylate proteins containing a C-terminal CaaX-box amino acid sequence with various modified isoprenoids. Here, we describe the design, synthesis, and application of a triorthogonal reagent, 1, that can be used to site-specifically incorporate an alkyne and aldehyde group simultaneously into a protein. To illustrate the capabilities of this approach, a protein was enzymatically modified with compound 1 followed by oxime ligation and click reaction to simultaneously incorporate an azido-tetramethylrhodamine (TAMRA) fluorophore and an aminooxy-PEG moiety. This was performed with both a model protein [green fluorescent protein (GFP)] as well as a therapeutically useful protein [ciliary neurotrophic factor (CNTF)]. Next, a protein was enzymatically modified with compound 1 followed by coupling to an azido-bis-methotrexate dimerizer and aminooxy-TAMRA. Incubation of that construct with a dihydrofolate reductase (DHFR)-DHFR-anti-CD3 fusion protein resulted in the self-assembly of nanoring structures that were endocytosed into T-leukemia cells and visualized therein. These results highlight how complex multifunctional protein assemblies can be prepared using this facile triorthogonal approach.

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Year:  2013        PMID: 24134212      PMCID: PMC3873327          DOI: 10.1021/ja403813b

Source DB:  PubMed          Journal:  J Am Chem Soc        ISSN: 0002-7863            Impact factor:   15.419


  45 in total

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4.  Chemically controlled self-assembly of protein nanorings.

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Review 5.  Site-specific labeling of proteins with small molecules in live cells.

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9.  A highly efficient catalyst for oxime ligation and hydrazone-oxime exchange suitable for bioconjugation.

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  18 in total

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5.  Simultaneous Site-Specific Dual Protein Labeling Using Protein Prenyltransferases.

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Review 7.  Recent progress in enzymatic protein labelling techniques and their applications.

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8.  Efficient farnesylation of an extended C-terminal C(x)3X sequence motif expands the scope of the prenylated proteome.

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10.  Engineering reversible cell-cell interactions using enzymatically lipidated chemically self-assembled nanorings.

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