Lang, Thorsten

[["dc.bibliographiccitation.firstpage","1072"],["dc.bibliographiccitation.issue","5841"],["dc.bibliographiccitation.journal","Science"],["dc.bibliographiccitation.lastpage","1076"],["dc.bibliographiccitation.volume","317"],["dc.contributor.author","Sieber, Jochen J."],["dc.contributor.author","Willig, Katrin I."],["dc.contributor.author","Kutzner, Carsten"],["dc.contributor.author","Gerding-Reimers, Claas"],["dc.contributor.author","Harke, Benjamin"],["dc.contributor.author","Donnert, Gerald"],["dc.contributor.author","Rammner, Burkhard"],["dc.contributor.author","Eggeling, Christian"],["dc.contributor.author","Hell, Stefan"],["dc.contributor.author","Grubmüller, Helmut"],["dc.contributor.author","Lang, Thorsten"],["dc.date.accessioned","2017-09-07T11:49:26Z"],["dc.date.available","2017-09-07T11:49:26Z"],["dc.date.issued","2007"],["dc.description.abstract","Most plasmalemmal proteins organize in submicrometer-sized clusters whose architecture and dynamics are still enigmatic. With syntaxin 1 as an example, we applied a combination of far-field optical nanoscopy, biochemistry, fluorescence recovery after photobleaching (FRAP) analysis, and simulations to show that clustering can be explained by self-organization based on simple physical principles. On average, the syntaxin clusters exhibit a diameter of 50 to 60 nanometers and contain 75 densely crowded syntaxins that dynamically exchange with freely diffusing molecules. Self-association depends on weak homophilic protein-protein interactions. Simulations suggest that clustering immobilizes and conformationally constrains the molecules. Moreover, a balance between self-association and crowding-induced steric repulsions is sufficient to explain both the size and dynamics of syntaxin clusters and likely of many oligomerizing membrane proteins that form supramolecular structures."],["dc.identifier.doi","10.1126/science.1141727"],["dc.identifier.gro","3143450"],["dc.identifier.isi","000248946700042"],["dc.identifier.pmid","17717182"],["dc.identifier.uri","https://resolver.sub.uni-goettingen.de/purl?gro-2/965"],["dc.language.iso","en"],["dc.notes.intern","WoS Import 2017-03-10"],["dc.notes.status","final"],["dc.notes.submitter","PUB_WoS_Import"],["dc.relation.issn","0036-8075"],["dc.title","Anatomy and dynamics of a supramolecular membrane protein cluster"],["dc.type","journal_article"],["dc.type.internalPublication","yes"],["dc.type.peerReviewed","yes"],["dc.type.subtype","original"],["dspace.entity.type","Publication"]]

[["dc.bibliographiccitation.firstpage","2843"],["dc.bibliographiccitation.issue","8"],["dc.bibliographiccitation.journal","Biophysical Journal"],["dc.bibliographiccitation.lastpage","2851"],["dc.bibliographiccitation.volume","90"],["dc.contributor.author","Sieber, Jochen J."],["dc.contributor.author","Willig, Katrin I."],["dc.contributor.author","Heintzmann, Rainer"],["dc.contributor.author","Hell, Stefan"],["dc.contributor.author","Lang, Thorsten"],["dc.date.accessioned","2017-09-07T11:53:10Z"],["dc.date.available","2017-09-07T11:53:10Z"],["dc.date.issued","2006"],["dc.description.abstract","In the plasma membrane, syntaxin 1 and syntaxin 4 clusters de. ne sites at which secretory granules and caveolae fuse, respectively. It is widely believed that lipid phases are mandatory for cluster formation, as cluster integrity depends on cholesterol. Here we report that the native lipid environment is not sufficient for correct syntaxin 1 clustering and that additional cytoplasmic protein-protein interactions, primarily involving the SNARE motif, are required. Apparently no specific cofactors are needed because i\\), clusters form equally well in nonneuronal cells, and ii\\), as revealed by nanoscale subdiffraction resolution provided by STED microscopy, the number of clusters directly depends on the syntaxin 1 concentration. For syntaxin 4 clustering the N-terminal domain and the linker region are also dispensable. Moreover, clustering is specific because in both cluster types syntaxins mutually exclude one another at endogenous levels. We suggest that the SNARE motifs of syntaxin 1 and 4 mediate specific syntaxin clustering by homooligomerization, thereby spatially separating sites for different biological activities. Thus, syntaxin clustering represents a mechanism of membrane patterning that is based on protein-protein interactions."],["dc.identifier.doi","10.1529/biophysj.105.079574"],["dc.identifier.gro","3143708"],["dc.identifier.isi","000236226900019"],["dc.identifier.pmid","16443657"],["dc.identifier.uri","https://resolver.sub.uni-goettingen.de/purl?gro-2/1252"],["dc.language.iso","en"],["dc.notes.intern","WoS Import 2017-03-10"],["dc.notes.status","final"],["dc.notes.submitter","PUB_WoS_Import"],["dc.relation.issn","0006-3495"],["dc.title","The SNARE motif is essential for the formation of syntaxin clusters in the plasma membrane"],["dc.type","journal_article"],["dc.type.internalPublication","yes"],["dc.type.peerReviewed","yes"],["dc.type.subtype","original"],["dspace.entity.type","Publication"]]

[["dc.bibliographiccitation.firstpage","3981"],["dc.bibliographiccitation.issue","17"],["dc.bibliographiccitation.journal","EMBO Journal"],["dc.bibliographiccitation.lastpage","3992"],["dc.bibliographiccitation.volume","26"],["dc.contributor.author","Bethani, Ioanna"],["dc.contributor.author","Lang, Thorsten"],["dc.contributor.author","Geumann, Ulf"],["dc.contributor.author","Sieber, Jochen J."],["dc.contributor.author","Jahn, Reinhard"],["dc.contributor.author","Rizzoli, Silvio"],["dc.date.accessioned","2017-09-07T11:49:25Z"],["dc.date.available","2017-09-07T11:49:25Z"],["dc.date.issued","2007"],["dc.description.abstract","Soluble N-ethylmaleimide-sensitive factor attachment receptor (SNARE) proteins mediate organelle fusion in the secretory pathway. Different fusion steps are catalyzed by specific sets of SNARE proteins. Here we have used the SNAREs mediating the fusion of early endosomes and exocytosis, respectively, to investigate how pairing specificity is achieved. Although both sets of SNAREs promiscuously assemble in vitro, there is no functional crosstalk. We now show that they not only colocalize to overlapping microdomains in the membrane of early endosomes of neuroendocrine cells, but also form cis-complexes promiscuously, with the proportion of the different complexes being primarily dependent on mass action. Addition of soluble SNARE molecules onto native membranes revealed preference for cognate SNAREs. Furthermore, we found that SNAREs are laterally segregated at endosome contact sites, with the exocytotic synaptobrevin being depleted. We conclude that specificity in endosome fusion is mediated by the following two synergistically operating mechanisms: (i) preference for the cognate SNARE in 'trans' interactions and (ii) lateral segregation of SNAREs, leading to relative enrichment of the cognate ones at the prospective fusion sites."],["dc.identifier.doi","10.1038/sj.emboj.7601820"],["dc.identifier.gro","3143442"],["dc.identifier.isi","000249691800010"],["dc.identifier.pmid","17717530"],["dc.identifier.uri","https://resolver.sub.uni-goettingen.de/purl?gro-2/956"],["dc.notes.intern","WoS Import 2017-03-10"],["dc.notes.status","final"],["dc.notes.submitter","PUB_WoS_Import"],["dc.publisher","Nature Publishing Group"],["dc.relation.issn","0261-4189"],["dc.title","The specificity of SNARE pairing in biological membranes is mediated by both proof-reading and spatial segregation"],["dc.type","journal_article"],["dc.type.internalPublication","yes"],["dc.type.peerReviewed","yes"],["dc.type.subtype","original"],["dspace.entity.type","Publication"]]