Now showing 1 - 3 of 3
  • 2018Journal Article
    [["dc.bibliographiccitation.artnumber","219"],["dc.bibliographiccitation.issue","1"],["dc.bibliographiccitation.journal","Scientific Reports"],["dc.bibliographiccitation.volume","8"],["dc.contributor.author","Wegner, Waja"],["dc.contributor.author","Mott, Alexander C."],["dc.contributor.author","Grant, Seth G. N."],["dc.contributor.author","Steffens, Heinz"],["dc.contributor.author","Willig, Katrin I."],["dc.date.accessioned","2019-07-09T11:45:13Z"],["dc.date.available","2019-07-09T11:45:13Z"],["dc.date.issued","2018"],["dc.description.abstract","The post-synaptic density (PSD) is an electron dense region consisting of ~1000 proteins, found at the postsynaptic membrane of excitatory synapses, which varies in size depending upon synaptic strength. PSD95 is an abundant scaffolding protein in the PSD and assembles a family of supercomplexes comprised of neurotransmitter receptors, ion channels, as well as signalling and structural proteins. We use superresolution STED (STimulated Emission Depletion) nanoscopy to determine the size and shape of PSD95 in the anaesthetised mouse visual cortex. Adult knock-in mice expressing eGFP fused to the endogenous PSD95 protein were imaged at time points from 1 min to 6 h. Superresolved large assemblies of PSD95 show different sub-structures; most large assemblies were ring-like, some horse-shoe or figure-8 shaped, and shapes were continuous or made up of nanoclusters. The sub-structure appeared stable during the shorter (minute) time points, but after 1 h, more than 50% of the large assemblies showed a change in sub-structure. Overall, these data showed a sub-morphology of large PSD95 assemblies which undergo changes within the 6 hours of observation in the anaesthetised mouse."],["dc.identifier.doi","10.1038/s41598-017-18640-z"],["dc.identifier.pmid","29317733"],["dc.identifier.purl","https://resolver.sub.uni-goettingen.de/purl?gs-1/15060"],["dc.identifier.uri","https://resolver.sub.uni-goettingen.de/purl?gro-2/59184"],["dc.language.iso","en"],["dc.notes.intern","Merged from goescholar"],["dc.relation","info:eu-repo/grantAgreement/EC/FP7/241498/EU//EUROSPIN"],["dc.relation.issn","2045-2322"],["dc.rights","CC BY 4.0"],["dc.rights.uri","https://creativecommons.org/licenses/by/4.0"],["dc.subject.ddc","610"],["dc.title","In vivo STED microscopy visualizes PSD95 sub-structures and morphological changes over several hours in the mouse visual cortex."],["dc.type","journal_article"],["dc.type.internalPublication","yes"],["dc.type.version","published_version"],["dspace.entity.type","Publication"]]
    Details DOI PMID PMC
  • 2021Journal Article Research Paper
    [["dc.bibliographiccitation.firstpage","eabf2806"],["dc.bibliographiccitation.issue","24"],["dc.bibliographiccitation.journal","Science Advances"],["dc.bibliographiccitation.volume","7"],["dc.contributor.author","Steffens, Heinz"],["dc.contributor.author","Mott, Alexander C."],["dc.contributor.author","Li, Siyuan"],["dc.contributor.author","Wegner, Waja"],["dc.contributor.author","Å vehla, Pavel"],["dc.contributor.author","Kan, Vanessa W. Y."],["dc.contributor.author","Wolf, Fred"],["dc.contributor.author","Liebscher, Sabine"],["dc.contributor.author","Willig, Katrin I."],["dc.date.accessioned","2021-07-05T14:57:45Z"],["dc.date.available","2021-07-05T14:57:45Z"],["dc.date.issued","2021"],["dc.description.abstract","Excitatory synapses on dendritic spines of pyramidal neurons are considered a central memory locus. To foster both continuous adaption and the storage of long-term information, spines need to be plastic and stable at the same time. Here, we advanced in vivo STED nanoscopy to superresolve distinct features of spines (head size and neck length/width) in mouse neocortex for up to 1 month. While LTP-dependent changes predict highly correlated modifications of spine geometry, we find both, uncorrelated and correlated dynamics, indicating multiple independent drivers of spine remodeling. The magnitude of this remodeling suggests substantial fluctuations in synaptic strength. Despite this high degree of volatility, all spine features exhibit persistent components that are maintained over long periods of time. Furthermore, chronic nanoscopy uncovers structural alterations in the cortex of a mouse model of neurodegeneration. Thus, at the nanoscale, stable dendritic spines exhibit a delicate balance of stability and volatility."],["dc.identifier.doi","10.1126/sciadv.abf2806"],["dc.identifier.pmid","34108204"],["dc.identifier.uri","https://resolver.sub.uni-goettingen.de/purl?gro-2/87727"],["dc.identifier.url","https://mbexc.uni-goettingen.de/literature/publications/265"],["dc.language.iso","en"],["dc.notes.intern","DOI-Import GROB-441"],["dc.relation","EXC 2067: Multiscale Bioimaging"],["dc.relation.eissn","2375-2548"],["dc.relation.workinggroup","RG Willig (Optical Nanoscopy in Neuroscience)"],["dc.relation.workinggroup","RG Wolf"],["dc.rights","CC BY-NC 4.0"],["dc.title","Stable but not rigid: Chronic in vivo STED nanoscopy reveals extensive remodeling of spines, indicating multiple drivers of plasticity"],["dc.type","journal_article"],["dc.type.internalPublication","yes"],["dc.type.subtype","original_ja"],["dc.type.version","published_version"],["dspace.entity.type","Publication"]]
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  • 2017-09-18Journal Article
    [["dc.bibliographiccitation.artnumber","11781"],["dc.bibliographiccitation.firstpage","1"],["dc.bibliographiccitation.issue","1"],["dc.bibliographiccitation.journal","Scientific reports"],["dc.bibliographiccitation.lastpage","10"],["dc.bibliographiccitation.volume","7"],["dc.contributor.author","Wegner, Waja"],["dc.contributor.author","Ilgen, Peter"],["dc.contributor.author","Gregor, Carola"],["dc.contributor.author","van Dort, Joris"],["dc.contributor.author","Mott, Alexander C."],["dc.contributor.author","Steffens, Heinz"],["dc.contributor.author","Willig, Katrin I."],["dc.date.accessioned","2019-07-09T11:44:29Z"],["dc.date.available","2019-07-09T11:44:29Z"],["dc.date.issued","2017-09-18"],["dc.description.abstract","The study of proteins in dendritic processes within the living brain is mainly hampered by the diffraction limit of light. STED microscopy is so far the only far-field light microscopy technique to overcome the diffraction limit and resolve dendritic spine plasticity at superresolution (nanoscopy) in the living mouse. After having tested several far-red fluorescent proteins in cell culture we report here STED microscopy of the far-red fluorescent protein mNeptune2, which showed best results for our application to superresolve actin filaments at a resolution of ~80 nm, and to observe morphological changes of actin in the cortex of a living mouse. We illustrate in vivo far-red neuronal actin imaging in the living mouse brain with superresolution for time periods of up to one hour. Actin was visualized by fusing mNeptune2 to the actin labels Lifeact or Actin-Chromobody. We evaluated the concentration dependent influence of both actin labels on the appearance of dendritic spines; spine number was significantly reduced at high expression levels whereas spine morphology was normal at low expression."],["dc.identifier.doi","10.1038/s41598-017-11827-4"],["dc.identifier.pmid","28924236"],["dc.identifier.purl","https://resolver.sub.uni-goettingen.de/purl?gs-1/14798"],["dc.identifier.uri","https://resolver.sub.uni-goettingen.de/purl?gro-2/59023"],["dc.language.iso","en"],["dc.notes.intern","Merged from goescholar"],["dc.relation.issn","2045-2322"],["dc.rights","CC BY 4.0"],["dc.rights.uri","https://creativecommons.org/licenses/by/4.0"],["dc.subject.ddc","573"],["dc.subject.ddc","612"],["dc.title","In vivo mouse and live cell STED microscopy of neuronal actin plasticity using far-red emitting fluorescent proteins."],["dc.type","journal_article"],["dc.type.internalPublication","yes"],["dc.type.version","published_version"],["dspace.entity.type","Publication"]]
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