Controlled Peptide-Mediated Vesicle Fusion Assessed by Simultaneous Dual-Colour Time-Lapsed Fluorescence Microscopy

Lopez Mora, N.; Boyle, A. L.; van Kolck, B. J.; Rossen, A.; Pokorná, Šárka; Koukalová, Alena; Šachl, Radek; Hof, Martin; Kros, A.

doi:https://dx.doi.org/10.1038/s41598-020-59926-z

Number of the records: 1

Controlled Peptide-Mediated Vesicle Fusion Assessed by Simultaneous Dual-Colour Time-Lapsed Fluorescence Microscopy

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SYSNO ASEP	0522602
Document Type	J - Journal Article
R&D Document Type	Journal Article
Subsidiary J	Článek ve WOS
Title	Controlled Peptide-Mediated Vesicle Fusion Assessed by Simultaneous Dual-Colour Time-Lapsed Fluorescence Microscopy
Author(s)	Lopez Mora, N. (NL) Boyle, A. L. (NL) van Kolck, B. J. (NL) Rossen, A. (NL) Pokorná, Šárka (UFCH-W)_RID Koukalová, Alena (UFCH-W)_RID Šachl, Radek (UFCH-W)_{RID, ORCID} Hof, Martin (UFCH-W)_{RID, ORCID} Kros, A. (NL)
Article number	3087
Source Title	Scientific Reports. - : Nature Publishing Group - ISSN 2045-2322 Roč. 10, č. 1 (2020)
Number of pages	13 s.
Language	eng - English
Country	GB - United Kingdom
Keywords	liposomes ; membrane fusion ; peptides
Subject RIV	CF - Physical ; Theoretical Chemistry
OECD category	Physical chemistry
R&D Projects	GA18-04871S GA ČR - Czech Science Foundation (CSF)
	GX19-26854X GA ČR - Czech Science Foundation (CSF)
Method of publishing	Open access
Institutional support	UFCH-W - RVO:61388955
UT WOS	000549177700001
EID SCOPUS	85079777213
DOI	10.1038/s41598-020-59926-z
Annotation	We have employed a model system, inspired by SnARe proteins, to facilitate membrane fusion between Giant Unilamellar Vesicles (GUVs) and Large Unilamellar Vesicles (LUVs) under physiological conditions. in this system, two synthetic lipopeptide constructs comprising the coiled-coil heterodimer-forming peptides K4, (KiAALKe)4, or e4, (eiAALeK)4, a peG spacer of variable length, and a cholesterol moiety to anchor the peptides into the liposome membrane replace the natural SnARe proteins. GUVs are functionalized with one of the lipopeptide constructs and the fusion process is triggered by adding LUVs bearing the complementary lipopeptide. Dual-colour time lapse fluorescence microscopy was used to visualize lipid- and content-mixing. Using conventional confocal microscopy, lipid mixing was observed on the lipid bilayer of individual GUVs. in addition to lipid-mixing, content-mixing assays showed a low efficiency due to clustering of K4-functionalized LUVs on the GUVs target membranes. We showed that, through the use of the non-ionic surfactant Tween 20, content-mixing between GUVs and LUVs could be improved, meaning this system has the potential to be employed for drug delivery in biological systems.
Workplace	J. Heyrovsky Institute of Physical Chemistry
Contact	Michaela Knapová, michaela.knapova@jh-inst.cas.cz, Tel.: 266 053 196
Year of Publishing	2021
Electronic address	http://hdl.handle.net/11104/0307069

Number of the records: 1