TY - JOUR A1 - Subramanian, Hariharan A1 - Döring, Frank A1 - Kollert, Sina A1 - Rukoyatkina, Natalia A1 - Sturm, Julia A1 - Gambaryan, Stepan A1 - Stellzig-Eisenhauer, Angelika A1 - Meyer-Marcotty, Philipp A1 - Eigenthaler, Martin A1 - Wischmeyer, Erhard T1 - PTH1R Mutants Found in Patients with Primary Failure of Tooth Eruption Disrupt G-Protein Signaling JF - PLoS One N2 - Aim Primary failure of tooth eruption (PFE) is causally linked to heterozygous mutations of the parathyroid hormone receptor (PTH1R) gene. The mutants described so far lead to exchange of amino acids or truncation of the protein that may result in structural changes of the expressed PTH1R. However, functional effects of these mutations have not been investigated yet. Materials and Methods In HEK293 cells, PTH1R wild type was co-transfected with selected PTH1R mutants identified in patients with PFE. The effects on activation of PTH-regulated intracellular signaling pathways were analyzed by ELISA and Western immunoblotting. Differential effects of wild type and mutated PTH1R on TRESK ion channel regulation were analyzed by electrophysiological recordings in Xenopus laevis oocytes. Results In HEK293 cells, activation of PTH1R wild type increases cAMP and in response activates cAMP-stimulated protein kinase as detected by phosphorylation of the vasodilator stimulated phosphoprotein (VASP). In contrast, the PTH1R mutants are functionally inactive and mutant PTH1R/Gly452Glu has a dominant negative effect on the signaling of PTH1R wild type. Confocal imaging revealed that wild type PTH1R is expressed on the cell surface, whereas PTH1R/Gly452Glu mutant is mostly retained inside the cell. Furthermore, in contrast to wild type PTH1R which substantially augmented K+ currents of TRESK channels, coupling of mutated PTH1R to TRESK channels was completely abolished. Conclusions PTH1R mutations affect intracellular PTH-regulated signaling in vitro. In patients with primary failure of tooth eruption defective signaling of PTH1R mutations is suggested to occur in dento-alveolar cells and thus may lead to impaired tooth movement. KW - phosphorylation KW - xenopus oocytes KW - calcium signaling KW - intracellular receptors KW - mutation KW - teeth KW - tooth eruption KW - transfection Y1 - 2016 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-147967 VL - 11 IS - 11 ER - TY - JOUR A1 - Stölting, Miriam A1 - Wiesner, Christiane A1 - van Vliet, Vanessa A1 - Butt, Elke A1 - Pavenstädt, Hermann A1 - Linder, Stefan A1 - Kremerskothen, Joachim T1 - Lasp-1 Regulates Podosome Function JF - PLoS One N2 - Eukaryotic cells form a variety of adhesive structures to connect with their environment and to regulate cell motility. In contrast to classical focal adhesions, podosomes, highly dynamic structures of different cell types, are actively engaged in matrix remodelling and degradation. Podosomes are composed of an actin-rich core region surrounded by a ring-like structure containing signalling molecules, motor proteins as well as cytoskeleton-associated proteins. Lasp-1 is a ubiquitously expressed, actin-binding protein that is known to regulate cytoskeleton architecture and cell migration. This multidomain protein is predominantely present at focal adhesions, however, a second pool of Lasp-1 molecules is also found at lamellipodia and vesicle-like microdomains in the cytosol. In this report, we show that Lasp-1 is a novel component and regulator of podosomes. Immunofluorescence studies reveal a localization of Lasp-1 in the podosome ring structure, where it colocalizes with zyxin and vinculin. Life cell imaging experiments demonstrate that Lasp-1 is recruited in early steps of podosome assembly. A siRNA-mediated Lasp-1 knockdown in human macrophages affects podosome dynamics as well as their matrix degradation capacity. In summary, our data indicate that Lasp-1 is a novel component of podosomes and is involved in the regulation of podosomal function. KW - discrete KW - smooth muscle cells KW - microdomains KW - actin cytoskeleton KW - endothelial cells KW - epithelial cells KW - cancer cells KW - phosphorylation KW - invadopodia KW - dependent protein-kinase KW - camp signaling pathway Y1 - 2012 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-134315 VL - 7 IS - 4 ER - TY - JOUR A1 - Navdaev, Alexey A1 - Subramanian, Hariharan A1 - Petunin, Alexey A1 - Clemetson, Kenneth J. A1 - Gambaryan, Stepan A1 - Walter, Ulrich T1 - Echicetin Coated Polystyrene Beads: A Novel Tool to Investigate GPIb-Specific Platelet Activation and Aggregation JF - PLoS ONE N2 - von Willebrand factor/ristocetin (vWF/R) induces GPIb-dependent platelet agglutination and activation of αIIbβ3 integrin, which also binds vWF. These conditions make it difficult to investigate GPIb-specific signaling pathways in washed platelets. Here, we investigated the specific mechanisms of GPIb signaling using echicetin-coated polystyrene beads, which specifically activate GPIb. We compared platelet activation induced by echicetin beads to vWF/R. Human platelets were stimulated with polystyrene beads coated with increasing amounts of echicetin and platelet activation by echicetin beads was then investigated to reveal GPIb specific signaling. Echicetin beads induced αIIbβ3-dependent aggregation of washed platelets, while under the same conditions vWF/R treatment led only to αIIbβ3-independent platelet agglutination. The average distance between the echicetin molecules on the polystyrene beads must be less than 7 nm for full platelet activation, while the total amount of echicetin used for activation is not critical. Echicetin beads induced strong phosphorylation of several proteins including p38, ERK and PKB. Synergistic signaling via P2Y12 and thromboxane receptor through secreted ADP and TxA2, respectively, were important for echicetin bead triggered platelet activation. Activation of PKG by the NO/sGC/cGMP pathway inhibited echicetin bead-induced platelet aggregation. Echicetin-coated beads are powerful and reliable tools to study signaling in human platelets activated solely via GPIb and GPIb-triggered pathways. KW - tyrosine KW - ERK signaling cascade KW - integrins KW - phosphorylation KW - polystyrene KW - platelet activation KW - platelet aggregation KW - platelets Y1 - 2014 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-119815 SN - 1932-6203 VL - 9 IS - 4 ER - TY - THES A1 - Mihlan, Sabrina [geb. Jasper] T1 - Identifikation von Zonula Occludens 2 (ZO-2) als neuen LASP-1 Interaktionspartner und Aufklärung der LASP-1/ZO-2 Kern-Zytosol Translokation T1 - Identification of zonula occludens 2 (ZO-2) as a new LASP-1binding partner and the elucidation of LASP-1/ZO-2 nucleo-cytoplasmatic shuttling N2 - LASP-1 (LIM und SH3 Domänen Protein) ist ein in Zellen ubiquitär vorkommendes Protein, welches in verschiedenen Tumorgeweben eine pathophysiologische Überexpression aufweist. Das Protein besitzt eine LIM Domäne, zwei Aktinbindungsregionen sowie eine SH3 Domäne und bindet einerseits an dynamischen Aktinstrukturen wie den fokalen Kontakten, Lamellopodien und Membranfortsätzen, kann andererseits aber auch in den Zellkern translokalisieren. Für Aktinstrukturen wirkt LASP-1 als Gerüstprotein und ist wichtig für die Migration und Proliferation der Zellen. Die Funktion von LASP-1 im Zellkern ist noch nicht bekannt, da aber in Tumorzellen eine erhöhte nukleare Akkumulation von LASP-1 beobachtet werden konnte, deren Intensität mit der Tumorgröße sowie dem Langzeitüberleben der Patientinnen korreliert, ist LASP-1, zusätzlich zu seiner Funktion als Strukturprotein, vermutlich auch ein Transkriptionsfaktor oder ein transkriptioneller Kofaktor. Eine Herunterregulation von LASP-1 in verschiedenen Tumorentitäten führt zur Inhibition der Proliferation und Migration. In dieser Arbeit konnte der bisher unbekannte Zellkernimport und -export von LASP-1 aufgeklärt werden. Maßgeblich daran beteiligt ist ein durch Pulldown Experimente neu identifizierter LASP-1 Bindungspartner: das Zonula Occludens 2 Protein (ZO-2). Mittels Immunpräzipitationen und Immunfluoreszenzen wurde diese Interaktion bestätigt. Nach Phosphorylierung von LASP-1 an Ser-146 durch Aktivierung der cAMP-abhängigen Proteinkinase (PKA) kommt es zu einer partiellen Ablösung des LASP-1/ZO-2 Komplexes aus den fokalen Kontakten hin zu einer vermehrten Kernlokalisation beider Proteine. Dies lässt sich durch Kern/Zytosol Trennungen belegen. Dabei ist die Bindung von LASP-1 an ZO-2 essentiell für die Translokation in den Zellkern, da bei einem ZO-2 Knockdown auch nach PKA Aktivierung LASP-1 zytosolisch lokalisiert bleibt. Wie Mutationsanalysen zeigen, findet die Interaktion zwischen der C-terminalen SH3 Domäne im LASP-1 und der Prolin-reichen SH3-Bindungssequenz im Bereich der Aminosäuren 1103-1121 am C-Terminus im ZO-2 statt. Die Translokation des Komplexes in den Kern erfolgt dabei über das Kernlokalisationssignal im ZO-2, da die LASP-1 Sequenz selbst keine nukleare Importsequenz aufweist. Im Zellkern konnte die direkte Interaktion von LASP-1 und ZO-2 mittels Duolink® Proximity Ligation Assay sichtbar gemacht werden. Der Export der Proteine erfolgt über das Protein CRM1. Eine Inhibition der Kernexportmaschinerie mit Leptomycin B erhöht die Konzentration beider Proteine im Zellkern. Das nukleare Exportsignal (NES) im LASP-1 konnte durch Punktmutationen N-terminal der Leucin-reichen Aminosäuresequenz 70-77 zugeordnet werden (NLRLKQQS). Im letzten Schritt dieses Zyklus erfolgt die Relokalisation von LASP-1 zurück an die Zellmembranstrukturen. Der neu gefundene Signalweg dient wahrscheinlich zur Weiterleitung von externen Stimuli in den Kern und zur Genregulation - mit LASP-1 als Transkriptionsfaktor oder transkriptionellen Kofaktor. N2 - LASP-1 (LIM and SH3 protein) is ubiquitously expressed at basal levels, but was found to be pathophysiologically overexpressed in several cancer entities. LASP-1 exhibits one LIM domain, two actin binding domains and one SH3 domain. On the one hand, LASP-1 is predominantly localized at focal contacts, lamellopodia and membrane ruffles, on the other hand a nuclear localization is observed. LASP-1 works as actin-binding scaffolding protein and is essential for migration and proliferation. Silencing of LASP-1 by RNA- interference in various cancer cell lines results in a strong inhibition of proliferation and migration. However, in tumor cells, an additional striking nuclear localization of the protein was observed, which significantly correlates with tumor size and a poor long term survival of the patients. Therefore, LASP-1 might act additionally as transcription factor or transcriptional co-factor In this work, a novel LASP-1 binding partner, zonula occludens protein 2 (ZO-2), was identified and its role in the signal transduction pathway of LASP-1 nucleo-cytoplasmic shuttling was established. Upon LASP-1 phosphorylation at Ser-146 by activated cAMP-dependent protein kinase A (PKA), LASP-1 binding to Zyxin and F-actin decreases and the protein detaches, in complex with ZO-2, from the plasma membrane and translocates into the nucleus. These results were confirmed by nuclear and cytosolic separation assays. Pull-down assays with mutants revealed that ZO-2 binds with its proline-rich sequence (amino acids 1103-1121) to the SH3 domain in LASP-1. LASP-1 exhibits no nuclear localization signal and requires ZO-2 to shuttle into the nucleus. In situ proximity ligation assay confirmed the direct binding between LASP-1 and ZO-2 and visualized the shuttling. Inhibition of the nuclear export system by Leptomycin B results in an accumulation of both proteins in nuclei. Nuclear export is regulated by the newly identified nuclear export signal in LASP-1 (amino acids 70-77) and mediated by CRM1. Finally LASP-1 relocalizes to focal contacts. This new identified pathway serves presumably as a signal transductor from the focal contacts to the nucleus for gene regulation. KW - Tumorzelle KW - Skleroproteine KW - Transkriptionsfaktor KW - Überexpression KW - Zellkern KW - Kern-Zytosoltranslokation KW - ZO-2 KW - Phosphorylierung KW - LASP-1 KW - nuclear cytosolic translocation KW - ZO-2 KW - phosphorylation Y1 - 2012 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-73442 ER -