High‐Speed Interferometric Scattering Tracking Microscopy of Compartmentalized Lipid Diffusion in Living Cells

dc.contributor.authorReina, Francesco
dc.contributor.authorEggeling, Christian
dc.contributor.authorLagerholm, Christoffer
dc.contributor.organizationfi=Turun biotiedekeskus|en=Turku Bioscience Centre|
dc.contributor.organization-code1.2.246.10.2458963.20.18586209670
dc.converis.publication-id504617930
dc.converis.urlhttps://research.utu.fi/converis/portal/Publication/504617930
dc.date.accessioned2026-01-21T12:43:00Z
dc.date.available2026-01-21T12:43:00Z
dc.description.abstractLateral diffusion measurements have been -used to infer information about the nano-organization of membranes. We employed interferometric scattering (ISCAT) microscopy at an acquisition rate of 2 kHz to revisit the diffusion dynamics of a phospholipid analog on the plasma membrane of Ptk2 cells. The ISCAT trajectory data are analyzed with an unbiased, statistics-driven pipeline to identify the most likely diffusion mode from a set of plausible diffusion modes. At the ensemble average level, the data are best described as transient compartmentalized diffusion with an average compartment size of 100-110 nm, transient confinement time of 8-10 ms, intracompartmental diffusion coefficient of 0.7-0.9 mu m2 s-1, and intercompartmental diffusion coefficient of 0.3-0.4 mu m2 s-1. The same analysis applied at the single-trajectory level identifies a complex variety of diffusion modes with 7-8% free, 13-14% confined, 40% transient compartmentalized, and 40% anomalous diffusion. Measurements with larger (& Oslash;40 nm) as compared to smaller (& Oslash;20 nm) gold nanoparticles are found to influence the diffusion rate and confinement strength, but not the underlying lipid diffusion modes. Using Monte Carlo simulations, these experimental results are explored in the wider context of relevant literature. This analysis paints a unifying picture of lipid diffusion on mammalian cell membranes transcending differences between experimental techniques.
dc.identifier.eissn1439-7641
dc.identifier.jour-issn1439-4235
dc.identifier.olddbid212882
dc.identifier.oldhandle10024/195900
dc.identifier.urihttps://www.utupub.fi/handle/11111/53899
dc.identifier.urlhttps://doi.org/10.1002/cphc.202400407
dc.identifier.urnURN:NBN:fi-fe202601217211
dc.language.isoen
dc.okm.affiliatedauthorLagerholm, Christoffer
dc.okm.discipline114 Physical sciencesen_GB
dc.okm.discipline116 Chemical sciencesen_GB
dc.okm.discipline3111 Biomedicineen_GB
dc.okm.discipline318 Medical biotechnologyen_GB
dc.okm.discipline114 Fysiikkafi_FI
dc.okm.discipline116 Kemiafi_FI
dc.okm.discipline3111 Biolääketieteetfi_FI
dc.okm.discipline318 Lääketieteen bioteknologiafi_FI
dc.okm.internationalcopublicationinternational co-publication
dc.okm.internationalityInternational publication
dc.okm.typeA1 ScientificArticle
dc.publisherWiley
dc.publisher.countryGermanyen_GB
dc.publisher.countrySaksafi_FI
dc.publisher.country-codeDE
dc.relation.articlenumbere202400407
dc.relation.doi10.1002/cphc.202400407
dc.relation.ispartofjournalChemPhysChem
dc.source.identifierhttps://www.utupub.fi/handle/10024/195900
dc.titleHigh‐Speed Interferometric Scattering Tracking Microscopy of Compartmentalized Lipid Diffusion in Living Cells
dc.year.issued2025

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