Vimentin levels and serine 71 phosphorylation in the control of cell-matrix adhesions, migration speed, and shape of transformed human fibroblasts

dc.bibliographicCitation.issue1eng
dc.bibliographicCitation.volume6
dc.contributor.authorTerriac, Emmanuel
dc.contributor.authorCoceano, Giovanna
dc.contributor.authorMavajian, Zahra
dc.contributor.authorHageman, Tijmen A.G.
dc.contributor.authorChrist, Andreas F.
dc.contributor.authorTesta, Ilaria
dc.contributor.authorLautenschläger, Franziska
dc.contributor.authorGad, Annica K.G.
dc.date.accessioned2018-04-04T09:13:10Z
dc.date.available2019-06-28T13:58:31Z
dc.date.issued2017
dc.description.abstractMetastasizing tumor cells show increased expression of the intermediate filament (IF) protein vimentin, which has been used to diagnose invasive tumors for decades. Recent observations indicate that vimentin is not only a passive marker for carcinoma, but may also induce tumor cell invasion. To clarify how vimentin IFs control cell adhesions and migration, we analyzed the nanoscale (30–50 nm) spatial organization of vimentin IFs and cell-matrix adhesions in metastatic fibroblast cells, using three-color stimulated emission depletion (STED) microscopy. We also studied whether wild-type and phospho-deficient or -mimicking mutants of vimentin changed the size and lifetime of focal adhesions (FAs), cell shape, and cell migration, using live-cell total internal reflection imaging and confocal microscopy. We observed that vimentin exists in fragments of different lengths. Short fragments were mostly the size of a unit-length filament and were mainly localized close to small cell-matrix adhesions. Long vimentin filaments were found in the proximity of large FAs. Vimentin expression in these cells caused a reduction in FAs size and an elongated cell shape, but did not affect FA lifetime, or the speed or directionality of cell migration. Expression of a phospho-mimicking mutant (S71D) of vimentin increased the speed of cell migration. Taken together, our results suggest that in highly migratory, transformed mesenchymal cells, vimentin levels control the cell shape and FA size, but not cell migration, which instead is linked to the phosphorylation status of S71 vimentin. These observations are consistent with the possibility that not only levels, but also the assembly status of vimentin control cell migration.eng
dc.description.versionpublishedVersioneng
dc.formatapplication/pdf
dc.identifier.urihttps://doi.org/10.34657/478
dc.identifier.urihttps://oa.tib.eu/renate/handle/123456789/4620
dc.language.isoengeng
dc.publisherBasel : MDPIeng
dc.relation.doihttps://doi.org/10.3390/cells6010002
dc.relation.ispartofseriesCells, Volume 6, Issue 1eng
dc.rights.licenseThis document may be downloaded, read, stored and printed for your own use within the limits of § 53 UrhG but it may not be distributed via the internet or passed on to external parties.eng
dc.rights.licenseDieses Dokument darf im Rahmen von § 53 UrhG zum eigenen Gebrauch kostenfrei heruntergeladen, gelesen, gespeichert und ausgedruckt, aber nicht im Internet bereitgestellt oder an Außenstehende weitergegeben werden.ger
dc.subjectfocal adhesionseng
dc.subjectvimentineng
dc.subjectcell migrationeng
dc.subjecttotal internal reflection (TIRF) microscopyeng
dc.subjectstimulated emission depletion (STED) microscopyeng
dc.subject.ddc570eng
dc.titleVimentin levels and serine 71 phosphorylation in the control of cell-matrix adhesions, migration speed, and shape of transformed human fibroblastseng
dc.typearticleeng
dc.typeTexteng
dcterms.bibliographicCitation.journalTitleCellseng
tib.accessRightsopenAccesseng
wgl.contributorINMeng
wgl.subjectBiowissenschaften/Biologieeng
wgl.typeZeitschriftenartikeleng
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