Literature DB >> 17315942

Protein-liposome conjugates using cysteine-lipids and native chemical ligation.

Sanne W A Reulen1, Wilco W T Brusselaars, Sander Langereis, Willem J M Mulder, Monica Breurken, Maarten Merkx.   

Abstract

Liposomes have become popular drug delivery vehicles and have more recently also been applied as contrast agents for molecular imaging. Most current methods for functionalization of liposomes with targeting proteins rely on reactions of amine or thiol groups at the protein exterior, which generally result in nonspecific conjugation at multiple sites on the protein. In this study, we present native chemical ligation (NCL) as a general method to covalently couple recombinant proteins in a highly specific and chemoselective way to liposomes containing cysteine-functionalized phospholipids. A cysteine-functionalized phospholipid (Cys-PEG-DSPE) was prepared and shown to readily react with the MESNA thioester of EYFP, which was used as a model protein. Characterization of the EYFP-liposomes using fluorescence spectroscopy showed full retention of the fluorescent properties of conjugated EYFP and provides a lower limit of 120 proteins per liposome. The general applicability of NCL was further tested using CNA35, a collagen-binding protein recently applied in fluorescent imaging of collagen. NCL of CNA35 thioester yielded liposomes containing approximately 100 copies of CNA35 per liposome. The CNA35-liposomes were shown to be fully functional and bind collagen with a 150-fold higher affinity compared to CNA35. Our results show that NCL is an attractive addition to existing conjugation methods that allows direct, covalent, and highly specific coupling of recombinant proteins to liposomes and other lipid-based assemblies.

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Year:  2007        PMID: 17315942     DOI: 10.1021/bc0602782

Source DB:  PubMed          Journal:  Bioconjug Chem        ISSN: 1043-1802            Impact factor:   4.774


  15 in total

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5.  Lipid modification of proteins through sortase-catalyzed transpeptidation.

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8.  Efficient, chemoselective synthesis of immunomicelles using single-domain antibodies with a C-terminal thioester.

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9.  Light-triggered sequence-specific cargo release from DNA block copolymer-lipid vesicles.

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Journal:  Mol Ther Nucleic Acids       Date:  2012-05-15       Impact factor: 10.183

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