Please use this identifier to cite or link to this item: http://hdl.handle.net/1942/42273
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dc.contributor.authorBACALUM, Mihaela-
dc.contributor.authorRADU, Mihai-
dc.contributor.authorOsella, Silvio-
dc.contributor.authorKNIPPENBERG, Stefan-
dc.contributor.authorAMELOOT, Marcel-
dc.date.accessioned2024-01-29T13:58:06Z-
dc.date.available2024-01-29T13:58:06Z-
dc.date.issued2024-
dc.date.submitted2024-01-12T14:34:16Z-
dc.identifier.citationJOURNAL OF PHOTOCHEMISTRY AND PHOTOBIOLOGY B-BIOLOGY, 250 (Art N° 112833)-
dc.identifier.issn1011-1344-
dc.identifier.urihttp://hdl.handle.net/1942/42273-
dc.description.abstractThe solvatochromic dye Laurdan is widely used in sensing the lipid packing of both model and biological membranes. The fluorescence emission maximum shifts from about 440 nm (blue channel) in condensed membranes (So) to about 490 nm (green channel) in the liquid-crystalline phase (Lα). Although the fluorescence intensity based generalized polarization (GP) is widely used to characterize lipid membranes, the fluorescence lifetime of Laurdan, in the blue and the green channel, is less used for that purpose. Here we explore the correlation between GP and fluorescence lifetimes by spectroscopic measurements on the So and Lα phases of large unilamellar vesicles of DMPC and DPPC. A positive correlation between GP and the lifetimes is observed in each of the optical channels for the two lipid phases. Microfluorimetric determinations on giant unilamellar vesicles of DPPC and DOPC at room temperature are performed under linearly polarized two-photon excitation to disentangle possible subpopulations of Laurdan at a scale below the optical resolution. Fluorescence intensities, GP and fluorescence lifetimes depend on the angle between the orientation of the linear polarization of the excitation light and the local normal to the membrane of the optical cross-section. This angular variation depends on the lipid phase and the emission channel. GP and fluorescence intensities in the blue and green channel in So and in the blue channel in Lα exhibit a minimum near 90o. Surprisingly, the intensity in the green channel in Lα reaches a maximum near 90o. The fluorescence lifetimes in the two optical channels also reach a pronounced minimum near 90o in So and Lα, apart from the lifetime in the blue channel in Lα where the lifetime is short with minimal angular variation. To our knowledge, these experimental observations are the first to demonstrate the existence of a bent conformation of Laurdan in lipid membranes, as previously suggested by molecular dynamics calculations.-
dc.description.sponsorshipThe authors are grateful to prof. L. Bagatolli for discussions at some point of this work, to Dr. N. Smisdom for advices regarding the use of the confocal microscope and data analysis of the confocal images and to Dr. R. Paesen for the home-made automated polarization controller device. The authors thank prof. M. Roeffaers for the ITO coated coverslips that were essential in the generation of GUV. S. O. is grateful to the National Science Centre, Poland for funding (grant no. UMO-2018/31/D/ST4/ 01475 and UMO/2020/39/I/ST4/01446). Computational time was at the Polish side provided by the Interdisciplinary Centre for Mathematical and Computational Modelling at the University of Warsaw (ICM UW) under grants no. G83-28 and GB80-24, while in Belgium the Flemish Supercomputer Centre (VSC) and the Herculesstichting are acknowledged.-
dc.language.isoen-
dc.publisherELSEVIER SCIENCE SA-
dc.rights2023 Elsevier B.V. All rights reserved.-
dc.subject.otherLaurdan-
dc.subject.otherGeneralized polarization-
dc.subject.otherFluorescence lifetimes-
dc.subject.otherAngular photoselectivity-
dc.subject.otherMicroheterogeneity-
dc.subject.otherConformational changes-
dc.titleGeneralized polarization and time-resolved fluorescence provide evidence for different populations of Laurdan in lipid vesicles-
dc.typeJournal Contribution-
dc.identifier.spage112833-
dc.identifier.volume250-
local.bibliographicCitation.jcatA1-
dc.description.notesAmeloot, M (corresponding author), Hasselt Univ, BIOMED, Agoralaan, B-3590 Diepenbeek, Belgium.-
dc.description.notesmarcel.ameloot@uhasselt.be-
local.publisher.placePO BOX 564, 1001 LAUSANNE, SWITZERLAND-
local.type.refereedRefereed-
local.type.specifiedArticle-
local.bibliographicCitation.artnr112833-
dc.identifier.doi10.1016/j.jphotobiol.2023.112833-
dc.identifier.pmid38141326-
dc.identifier.isi001147810800001-
dc.identifier.eissn1873-2682-
local.provider.typePdf-
local.description.affiliation[Bacalum, Mihaela; Radu, Mihai] Horia Hulubei Natl Inst Phys & Nucl Engn, Dept Life & Environm Phys, Reactorului 30, Magurele 077125, Romania.-
local.description.affiliation[Osella, Silvio] Univ Warsaw, Ctr New Technol, Chem & Biol Syst Simulat Lab, Banacha 2C, PL-02097 Warsaw, Poland.-
local.description.affiliation[Knippenberg, Stefan; Ameloot, Marcel] Hasselt Univ, Biomed Res Inst, Agoralaan Bldg C, B-3590 Diepenbeek, Belgium.-
local.description.affiliation[Knippenberg, Stefan] Hasselt Univ, Theory Lab, Agoralaan Bldg D, B-3590 Diepenbeek, Belgium.-
local.description.affiliation[Ameloot, Marcel] Hasselt Univ, BIOMED, Agoralaan, B-3590 Diepenbeek, Belgium.-
local.uhasselt.internationalyes-
item.fulltextWith Fulltext-
item.accessRightsEmbargoed Access-
item.embargoEndDate2024-07-01-
item.fullcitationBACALUM, Mihaela; RADU, Mihai; Osella, Silvio; KNIPPENBERG, Stefan & AMELOOT, Marcel (2024) Generalized polarization and time-resolved fluorescence provide evidence for different populations of Laurdan in lipid vesicles. In: JOURNAL OF PHOTOCHEMISTRY AND PHOTOBIOLOGY B-BIOLOGY, 250 (Art N° 112833).-
item.contributorBACALUM, Mihaela-
item.contributorRADU, Mihai-
item.contributorOsella, Silvio-
item.contributorKNIPPENBERG, Stefan-
item.contributorAMELOOT, Marcel-
crisitem.journal.issn1011-1344-
crisitem.journal.eissn1873-2682-
Appears in Collections:Research publications
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