Literature DB >> 18787836

Spatiotemporal analysis of endocytosis and membrane distribution of fluorescent sterols in living cells.

Daniel Wüstner1, Nils J Faergeman.   

Abstract

Distribution and dynamics of cholesterol in the plasma membrane as well as internalization pathways for sterol from the cell surface are of great cell biological interest. Here, UV-sensitive wide field microscopy of the intrinsically fluorescent sterols, dehydroergosterol (DHE) and cholestatrienol (CTL) combined with advanced image analysis were used to study spatiotemporal sterol distribution in living macrophages, adipocytes and fibroblasts. Sterol endocytosis was directly visualized by time-lapse imaging and noise-robust tracking revealing confined motion of DHE containing vesicles in close proximity to the cell membrane. Spatial surface intensity patterns of DHE as well as that of the lipid marker DiIC12 being assessed by statistical image analysis persisted over several minutes in cells having a constant overall curvature. Sites of sterol endocytosis appeared indistinguishable from other regions of the cell surface, and endocytosis contributed by 62% to total sterol uptake in J774 cells. DHE co-localized with fluorescent transferrin (Tf) in vesicles right after onset of endocytosis and in deepened surface patches of energy depleted cells. Surface caveolae labeled with GFP-tagged caveolin were not particularly enriched in DHE or CTL. Some sterol co-localized with internalized caveolin suggesting that caveolar endocytosis contributes to vesicular sterol uptake. These findings demonstrate that plasma membrane sterol is internalized by several endocytic pathways. Sterol endocytosis does not require formation of microscopically resolvable sterol clusters or enrichment of sterol in surface caveolae.

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Year:  2008        PMID: 18787836     DOI: 10.1007/s00418-008-0488-6

Source DB:  PubMed          Journal:  Histochem Cell Biol        ISSN: 0948-6143            Impact factor:   4.304


  58 in total

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4.  Caveolae are highly immobile plasma membrane microdomains, which are not involved in constitutive endocytic trafficking.

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5.  Direct observation of rapid internalization and intracellular transport of sterol by macrophage foam cells.

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Review 6.  Fluorescent sterols as tools in membrane biophysics and cell biology.

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7.  Chromatic aberration correction and deconvolution for UV sensitive imaging of fluorescent sterols in cytoplasmic lipid droplets.

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Journal:  Cytometry A       Date:  2008-08       Impact factor: 4.355

8.  Structure and cholesterol domain dynamics of an enriched caveolae/raft isolate.

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9.  The cholesterol absorption inhibitor ezetimibe acts by blocking the sterol-induced internalization of NPC1L1.

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3.  Analysis of cholesterol trafficking with fluorescent probes.

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6.  Two-photon time-lapse microscopy of BODIPY-cholesterol reveals anomalous sterol diffusion in chinese hamster ovary cells.

Authors:  Frederik W Lund; Michael A Lomholt; Lukasz M Solanko; Robert Bittman; Daniel Wüstner
Journal:  BMC Biophys       Date:  2012-10-18       Impact factor: 4.778

Review 7.  Fluorescent Sterols and Cholesteryl Esters as Probes for Intracellular Cholesterol Transport.

Authors:  Katarzyna A Solanko; Maciej Modzel; Lukasz M Solanko; Daniel Wüstner
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  7 in total

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