2013
DOI: 10.1021/ja4031227
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In Situ Modification of Plain Liposomes with Lipidated Coiled Coil Forming Peptides Induces Membrane Fusion

Abstract: Complementary coiled coil forming lipidated peptides embedded in liposomal membranes are able to induce rapid, controlled, and targeted membrane fusion. Traditionally, such fusogenic liposomes are prepared by mixing lipids and lipidated peptides in organic solvent (e.g., chloroform). Here we prepared fusogenic liposomes in situ, i.e., by addition of a lipidated peptide solution to plain liposomes. As the lipid anchor is vital for the correct insertion of lipidated peptides into liposomal membranes, a small lib… Show more

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Cited by 109 publications
(148 citation statements)
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“…Identity of the peptides was determined by liquid chromatography-mass spectrometry. The lipopeptides were synthesized and purified as described elsewhere (7,9). Peptide stock solutions in PBS were prepared~2 mg/ml and the concentration was determined by ultraviolet absorbance at 280 nm, for peptides without tryptophan the concentration was based on the mass.…”
Section: Peptide Synthesismentioning
confidence: 99%
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“…Identity of the peptides was determined by liquid chromatography-mass spectrometry. The lipopeptides were synthesized and purified as described elsewhere (7,9). Peptide stock solutions in PBS were prepared~2 mg/ml and the concentration was determined by ultraviolet absorbance at 280 nm, for peptides without tryptophan the concentration was based on the mass.…”
Section: Peptide Synthesismentioning
confidence: 99%
“…Fig. 2 A displays the change of fluorescence intensity upon varying the lipid to peptide ratio by addition of vesicles of the composition DOPC:DOPE:cholesterol (molar ratio: 2:1:1), as used in recent vesicle fusion studies (5)(6)(7)(8)(9)(10)16,44,45). For comparative purposes, the total concentration of the tryptophan bearing peptide (X*, X ¼ K or E, respectively) was kept constant.…”
Section: Membrane Binding Of K Before and After Vesicle Dockingmentioning
confidence: 99%
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“…The lipopeptides were analyzed by electrospray-ionization mass spectrometry (E3Cys-MCCDOPE: 3882 m z À1 [Mþ], K3Cys-MCCDOPE: 3827 m z À1 [Mþ]). Additionally, cholesterol-PEG12-E4 and cholesterol-PEG12-K4 were used to induce membrane fusion between the silica beads (10)(11)(12)(13). some experiments one fraction contained a different fluorescent dye lipid such as Oregon Green 488 DPPE, Atto488-DOPE, or ATTO390DOPE (1 mol %).…”
Section: Lipopeptidesmentioning
confidence: 99%
“…In order to enhance the intracellular delivery of MSNs/cytC, the nanoparticles were coated with a fusogenic lipid bilayer containing 1 mol% CP 4 E 4 (MSNs/cytC@CPE-LBs). To induce nanoparticle uptake via membrane fusion, cells were pretreated with CP 4 K 4 [29] and subsequently MSNs/cytC@CPE-LBs were added to the medium. Lipopeptides and lipid bilayer coated MSNs with or without CP 4 E 4 were well tolerated by HeLa cells as no signs of toxicity were observed ( Figure S2, Supporting Information).…”
Section: Intracellular Delivery Of Cytcmentioning
confidence: 99%