TY  - THES
A1  - Baljuls, Angela
T1  - Differences and Similarities in the Regulation of RAF Isoforms: Identification of Novel A-RAF Phosphorylation Sites
T1  - Unterschiede und Ähnlichkeiten in der Regulierung der RAF Isoformen : Identifizierung der neuen A-RAF Phosphorylierungsstellen
N2  - In mammals, the RAF family of serine/threonine kinases consists of three members, A-, B- and C-RAF. Activation of RAF kinases involves a complex series of phosphorylations. Although the most prominent phosphorylation sites of B- and C-RAF are well characterized, little is known about regulatory phosphorylation of A-RAF. Using mass spectrometry, we identified here a number of novel in vivo phosphorylation sites in A-RAF. The physiological role and the function of these sites were investigated subsequently by amino acid exchange at the relevant positions. In particular, we found that S432 participates in MEK binding and is indispensable for A-RAF signaling. On the other hand, phosphorylation within the activation segment does not contribute to epidermal growth factor-mediated activation. Regarding regulation of A-RAF activity by 14-3-3 proteins, we show that A-RAF activity is regulated differentially by its C-terminal and internal 14-3-3 binding domain. Furthermore, by use of SPR technique, we found that 14-3-3 proteins associate with RAF in an isoform-specific manner. Of importance, we identified a novel regulatory domain in A-RAF (referred to as IH-segment) positioned between amino acids 248 and 267, which contains seven putative phosphorylation sites. Three of these sites, serines 257, 262 and 264, regulate A-RAF activation in a stimulatory manner. The spatial model of the A-RAF fragment including residues between S246 and E277 revealed a “switch of charge” at the molecular surface of the IH-region upon phosphorylation, suggesting a mechanism in which the high accumulation of negative charges may lead to an electrostatic destabilization of protein/membrane interaction resulting in depletion of A-RAF from the plasma membrane. Activation of B- and C-RAF is regulated by phosphorylation at conserved residues within the negative-charge regulatory region (N-region). Identification of phosphopeptides covering the sequence of the N-region led to the conclusion that, similar to B- and C-RAF, kinase activity of A-RAF is regulated by phosphorylation of the N-region. Abrogation of A-RAF activity by S299A substitution and elevated activity of the A-RAF-Y301D-Y302D mutant confirmed this conclusion. In addition, we studied the role of the non-conserved residues within the N-region in the activation process of RAF kinases. The non-conserved amino acids in positions –3 and +1 relative to the highly conserved S299 in A-RAF and S338 in C-RAF have so far not been considered as regulatory residues. Here, we demonstrate that Y296R substitution in A-RAF led to a constitutively active kinase. In contrast, G300S substitution (mimicking B- and C-RAF) acts in an inhibitory manner. These data were confirmed by analogous mutations in C-RAF. Based on the three-dimensional structure of the catalytic domain of B-RAF, a tight interaction between the N-region residue S339 and the catalytic domain residue R398 was identified in C-RAF and proposed to inhibit the kinase activity of RAF proteins. Furthermore, Y296 in A-RAF favors a spatial orientation of the N-region segment, which enables a tighter contact to the catalytic domain, whereas a glutamine residue at this position in C-RAF abrogates this interaction. Considering this observation, we suggest that Y296, which is unique for A-RAF, is a major determinant of the low activating potency of this RAF isoform. Finally, the residues R359 in A-RAF and R398 in C-RAF, which interact with the N-region, are also involved in binding of phosphatidic acid. Substitution of this conserved arginine by alanine resulted in accumulation of hyper-phosphorylated form of RAF, suggesting that this residue play a crucial role in phosphorylation-mediated feedback regulation of A- and C-RAF. Collectively, we provide here for the first time a detailed analysis of in vivo A-RAF phosphorylation status and demonstrate that regulation of A-RAF by phosphorylation exhibits unique features compared with B- and C-RAF.
N2  - Die Protein-Familie der Serin/Threonin-spezifischen RAF-Kinasen umfasst in Säugetieren drei Mitglieder, A-, B- und C-RAF. Bei der Aktivierung dieser Kinasen spielen Phosphorylierungs-ereignisse eine entscheidende Rolle. Im Gegensatz zu B- und C-RAF, deren Phosphorylierungsstellen ausgiebig charakterisiert sind, blieb die Phosphorylierung von A-RAF weitgehend unerforscht. In der vorliegenden Arbeit wurden unter Verwendung der massenspektrometrischen Analyse zahlreiche neue in vivo A-RAF-Phosphorylierungsstellen identifiziert. Die physiologische Relevanz und die Funktion dieser Stellen wurden anschließend durch Aminosäurenaustausch an den relevanten Positionen untersucht. Dabei wurde festgestellt, dass S432 in der A-RAF-Bindung zu MEK involviert und für die Signalweiterleitung unverzichtbar ist. Hingegen ist die EGF-bedingte A-RAF-Aktivierung nicht von der Phosphorylierung innerhalb des Aktivierungssegments abhängig. Hinsichtlich der Regulation von A-RAF-Aktivierung durch 14-3-3-Proteine, wurde hier gezeigt, dass die katalytische Aktivität von A-RAF durch die C-terminale und die interne 14-3-3-Bindungsdomänen unterschiedlich reguliert wird. Weiterhin wurde mittels SPR-Verfahren festgestellt, dass die Interaktion von 14-3-3-Proteinen mit RAF-Kinasen einen isoformspezifischen Charakter trägt. Von entscheidender Bedeutung war die Entdeckung einer neuen regulatorischen Domäne (hier als IH-Segment bezeichnet), die in der A-RAF-Sequenz die Aminosäuren 248 bis 267 umfasst und sieben A-RAF-spezifische Phosphorylierungsstellen enthält. Drei dieser Stellen, S257, S262 und S264, erwiesen sich als positive Regulatoren der A-RAF-Aktivierung. Das räumliche Modell dieses A-RAF-Fragments deckte eine „Ladungsumkehr“ an der molekularen Oberfläche der IH-Region infolge der Phosphorylierung auf. Dieser Befund begründete den Vorschlag eines Regulations-mechanismus, in dem die starke Akkumulierung der negativen Ladungen zu einer elektrostatischen Destabilisierung der Protein-Membran-Interaktion führt, was die Verdrängung der A-RAF-Kinase von der Plasma-Membran zur Folge haben könnte. Die Aktivierung von B- und C-RAF wird durch Phosphorylierung der sogenannten „negativ geladenen“ Region (N-Region) reguliert. Die Identifizierung mehrerer Phosphopeptide aus der N-Region von A-RAF veranlasste die Schlussfolgerung, dass die A-RAF-Aktivität ebenfalls durch die Phosphorylierung innerhalb dieser Region gesteuert werden könnte. In der Tat, die Aufhebung der A-RAF-Aktivität durch die S299A-Substitution und die erhöhte Aktivität der A-RAF-Y301D-Y302D-Mutante bestätigen diese Aussage. Darüberhinaus wurde die Rolle der nichtkonservierten Aminosäuren an den Positionen –3 und +1 relativ zum S299 in A-RAF und S338 in C-RAF im Aktivierungsprozess der RAF-Kinasen untersucht, nachdem diese ursprünglich nicht als regulatorische Stellen erkannt wurden. Es wird hier demonstriert, dass Y296R-Substitution der A-RAF-Kinase eine konstitutive Aktivität verleiht. Hingegen wirkte die G300S-Substitution, die von B- und C-RAF abgeleitet wurde, inhibitorisch. Diese Befunde wurden durch die analogen Mutationen in C-RAF bestätigt. Basierend auf der dreidimensionalen Struktur der katalytischen Domäne von B-RAF wurde eine Interaktion zwischen der N-Region und der katalytischen Domäne in A- und C-RAF festgestellt, die zu einer Inhibierung der Aktivität führen soll. Darüberhinaus wurde gezeigt, dass die räumliche Ausrichtung von Y296 in der N-Region von A-RAF einen engen Kontakt mit der katalytischen Domäne ermöglicht; dagegen hebt Glutamin in dieser Position die Interaktion auf. In Anbetracht dieser Befunde wurde vorschlagen, dass das A-RAF-spezifische Y296 das niedrige Aktivierungs-potential dieser RAF-Isoform determiniert. In diesem Zusammenhang wurde auch gefunden, dass die Aminosäuren R359 in A-RAF und R398 in C-RAF eine duale Funktion besitzen, indem sie sowohl mit der N-Region als auch mit Lipiden in Wechselwirkung treten können. Substitution dieser konservierten Arginine durch Alanin führte zur Akkumulierung der hyperphosphorylierten Formen der RAF-Kinasen, was die Schlussfolgerung erlaubt, dass diese Reste eine wichtige Rolle in der ERK-vermittelten Feedback-Regulation von A- und C-RAF spielen. Insgesamt wird hier zum ersten Mal eine detaillierte Analyse der in vivo A-RAF-Phosphorylierung geliefert und gezeigt, dass die phosphorylierungsvermittelte Regulation von A-RAF einzigartige Merkmale innerhalb der Familie von RAF-Kinasen aufweist.
KW  - Raf <Biochemie>
KW  - Phosphorylierung
KW  - Signaltransduktion
KW  - RAF kinases
KW  - phosphorylation
KW  - signal trunsduction
Y1  - 2009
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-36135
ER  - 
TY  - JOUR
A1  - Dreyer, Ingo
A1  - Gomez-Porras, Judith Lucia
A1  - Riaño-Pachón, Diego Mauricio
A1  - Hedrich, Rainer
A1  - Geiger, Dietmar
T1  - Molecular Evolution of Slow and Quick Anion Channels (SLACs and QUACs/ALMTs)
JF  - Frontiers in Plant Science
N2  - Electrophysiological analyses conducted about 25 years ago detected two types of anion channels in the plasma membrane of guard cells. One type of channel responds slowly to changes in membrane voltage while the other responds quickly. Consequently, they were named SLAC, for SLow Anion Channel, and QUAC, for QUick Anion Channel. Recently, genes SLAC1 and QUAC1/ALMT12, underlying the two different anion current components, could be identified in the model plant Arabidopsis thaliana. Expression of the gene products in Xenopus oocytes confirmed the quick and slow current kinetics. In this study we provide an overview on our current knowledge on slow and quick anion channels in plants and analyze the molecular evolution of ALMT/QUAC-like and SLAC-like channels. We discovered fingerprints that allow screening databases for these channel types and were able to identify 192 (177 non-redundant) SLAC-like and 422 (402 non-redundant) ALMT/QUAC-like proteins in the fully sequenced genomes of 32 plant species. Phylogenetic analyses provided new insights into the molecular evolution of these channel types. We also combined sequence alignment and clustering with predictions of protein features, leading to the identification of known conserved phosphorylation sites in SLAC1-like channels along with potential sites that have not been yet experimentally confirmed. Using a similar strategy to analyze the hydropathicity of ALMT/QUAC-like channels, we propose a modified topology with additional transmembrane regions that integrates structure and function of these membrane proteins. Our results suggest that cross-referencing phylogenetic analyses with position-specific protein properties and functional data could be a very powerful tool for genome research approaches in general.
KW  - anion channel
KW  - evolution
KW  - SLAC/SLAH
KW  - ALMT
KW  - QUAC
KW  - voltage dependent
KW  - topology
KW  - phosphorylation
Y1  - 2012
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-189345
SN  - 1664-462X
VL  - 3
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  - Szabó, Áron
A1  - Papin, Christian
A1  - Zorn, Daniela
A1  - Ponien, Prishila
A1  - Weber, Frank
A1  - Raabe, Thomas
A1  - Rouyer, François
T1  - The CK2 Kinase Stabilizes CLOCK and Represses Its Activity in the Drosophila Circadian Oscillator
JF  - PLoS Biology
N2  - Phosphorylation is a pivotal regulatory mechanism for protein stability and activity in circadian clocks regardless of their evolutionary origin. It determines the speed and strength of molecular oscillations by acting on transcriptional activators and their repressors, which form negative feedback loops. In Drosophila, the CK2 kinase phosphorylates and destabilizes the PERIOD (PER) and TIMELESS (TIM) proteins, which inhibit CLOCK (CLK) transcriptional activity. Here we show that CK2 also targets the CLK activator directly. Downregulating the activity of the catalytic alpha subunit of CK2 induces CLK degradation, even in the absence of PER and TIM. Unexpectedly, the regulatory beta subunit of the CK2 holoenzyme is not required for the regulation of CLK stability. In addition, downregulation of \(CK2\alpha\) activity decreases CLK phosphorylation and increases per and tim transcription. These results indicate that CK2 inhibits CLK degradation while reducing its activity. Since the CK1 kinase promotes CLK degradation, we suggest that CLK stability and transcriptional activity result from counteracting effects of CK1 and CK2.
KW  - negative feedback loop
KW  - PER-TIM complex
KW  - posttranslational regulation
KW  - transcription factor
KW  - in-vivo
KW  - behavioral rhythms
KW  - proteins period
KW  - beta-subunit
KW  - phosphorylation
KW  - gene
KW  - CT, circadian time
KW  - LD, light:dark
KW  - DD, constant darkness
Y1  - 2013
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-127234
SN  - 1545-7885
VL  - 11
IS  - 8
ER  - 
TY  - JOUR
A1  - Rauert-Wunderlich, Hilka
A1  - Siegmund, Daniela
A1  - Maier, Eduard
A1  - Giner, Tina
A1  - Bargou, Ralf C.
A1  - Wajant, Harald
A1  - Stühmer, Thorsten
T1  - The IKK Inhibitor Bay 11-7082 Induces Cell Death Independent from Inhibition of Activation of NF kappa B Transcription Factors
JF  - PLoS ONE
N2  - Multiple myeloma (MM) displays an NFκB activity-related gene expression signature and about 20% of primary MM samples harbor genetic alterations conducive to intrinsic NFκB signaling activation. The relevance of blocking the classical versus the alternative NFκB signaling pathway and the molecular execution mechanisms involved, however, are still poorly understood. Here, we comparatively tested NFκB activity abrogation through TPCA-1 (an IKK2 inhibitor), BAY 11-7082 (an IKK inhibitor poorly selective for IKK1 and IKK2), and MLN4924 (an NEDD8 activating enzyme (NAE)-inhibitor), and analyzed their anti-MM activity. Whereas TPCA-1 interfered selectively with activation of the classical NFκB pathway, the other two compounds inhibited classical and alternative NFκB signaling without significant discrimination. Noteworthy, whereas TPCA-1 and MLN4924 elicited rather mild anti-MM effects with slight to moderate cell death induction after 1 day BAY 11-7082 was uniformly highly toxic to MM cell lines and primary MM cells. Treatment with BAY 11-7082 induced rapid cell swelling and its initial effects were blocked by necrostatin-1 or the ROS scavenger BHA, but a lasting protective effect was not achieved even with additional blockade of caspases. Because MLN4924 inhibits the alternative NFκB pathway downstream of IKK1 at the level of p100 processing, the quite discordant effects between MLN4924 and BAY 11-7082 must thus be due to blockade of IKK1-mediated NFκB-independent necrosis-inhibitory functions or represent an off-target effect of BAY 11-7082. In accordance with the latter, we further observed that concomitant knockdown of IKK1 and IKK2 did not have any major short-term adverse effect on the viability of MM cells.
KW  - signal inhibition
KW  - necrotic cell death
KW  - cell viability testing
KW  - cell death
KW  - small interfering RNAs
KW  - HT29 cells
KW  - phosphorylation
KW  - multiple myeloma
Y1  - 2013
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-130140
VL  - 8
IS  - 3
ER  - 
TY  - JOUR
A1  - Rudel, Thomas
A1  - Faulstich, Michaela
A1  - Böttcher, Jan-Peter
A1  - Meyer, Thomas F.
A1  - Fraunholz, Martin
T1  - Pilus Phase Variation Switches Gonococcal Adherence to Invasion by Caveolin-1-Dependent Host Cell Signaling
JF  - PLoS Pathogens
N2  - Many pathogenic bacteria cause local infections but occasionally invade into the blood stream, often with fatal outcome. Very little is known about the mechanism underlying the switch from local to invasive infection. In the case of Neisseria gonorrhoeae, phase variable type 4 pili (T4P) stabilize local infection by mediating microcolony formation and inducing anti-invasive signals. Outer membrane porin PorBIA, in contrast, is associated with disseminated infection and facilitates the efficient invasion of gonococci into host cells. Here we demonstrate that loss of pili by natural pilus phase variation is a prerequisite for the transition from local to invasive infection. Unexpectedly, both T4P-mediated inhibition of invasion and PorBIA-triggered invasion utilize membrane rafts and signaling pathways that depend on caveolin-1-Y14 phosphorylation (Cav1-pY14). We identified p85 regulatory subunit of PI3 kinase (PI3K) and phospholipase Cγ1 as new, exclusive and essential interaction partners for Cav1-pY14 in the course of PorBIA-induced invasion. Active PI3K induces the uptake of gonococci via a new invasion pathway involving protein kinase D1. Our data describe a novel route of bacterial entry into epithelial cells and offer the first mechanistic insight into the switch from local to invasive gonococcal infection.
KW  - antibodies
KW  - bacterial pathogens
KW  - cell membranes
KW  - intracellular pathogens
KW  - neisseria gonorrhoeae
KW  - phosphates
KW  - phosphorylation
KW  - pili and fimbriae
Y1  - 2013
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-96679
ER  - 
TY  - JOUR
A1  - Fehrholz, Markus
A1  - Christian P., Speer
A1  - Kunzmann, Steffen
T1  - Caffeine and Rolipram Affect Smad Signalling and TGFβ1 Stimulated CTGF and Transgelin Expression in Lung Epithelial Cells
JF  - PLoS One
N2  - Caffeine administration is an important part of the therapeutic treatment of bronchopulmonary dysplasia (BPD) in preterm infants. However, caffeine mediated effects on airway remodelling are still undefined. The TGF-β/Smad signalling pathway is one of the key pathways involved in airway remodelling. Connective tissue growth factor (CTGF), a downstream mediator of TGF-β, and transgelin, a binding and stabilising protein of the cytoskeleton, are both regulated by TGF-b1 and play an important role in airway remodelling. Both have also been implicated in the pathogenesis of BPD. The aim of the present study was to clarify whether caffeine, an unspecific phosphodiesterase (PDE) inhibitor, and rolipram, a prototypical PDE-4 selective inhibitor, were both able to affect TGF-β1-induced Smad signalling and CTGF/transgelin expression in lung epithelial cells. Furthermore, the effect of transgelin knock-down on Smad signalling was studied. The pharmacological effect of caffeine and rolipram on Smad signalling was investigated by means of a luciferase assay via transfection of a TGFβ1- inducible reporter plasmid in A549 cells. The regulation of CTGF and transgelin expression by caffeine and rolipram were studied by promoter analysis, real-time PCR and Western blot. Endogenous transgelin expression was down-regulated by lentiviral transduction mediating transgelin-specific shRNA expression. The addition of caffeine and rolipram inhibited TGFβ1 induced reporter gene activity in a concentration-related manner. They also antagonized the TGF-b1 induced upregulation of CTGF and transgelin on the promoter-, the mRNA-, and the protein-level. Functional analysis showed that transgelin silencing reduced TGF-β1 induced Smad-signalling and CTGF induction in lung epithelial cells. The present study highlights possible new molecular mechanisms of caffeine and rolipram including an inhibition of Smad signalling and of TGF-β1 regulated genes involved in airway remodelling. An understanding of these mechanisms might help to explain the protective effects of caffeine in prevention of BPD and suggests rolipram to be a potent replacement for caffeine.
KW  - caffein
KW  - SMAD signaling
KW  - epithelial cells
KW  - luciferase
KW  - DNA-binding proteins
KW  - immunoblotting
KW  - phosphorylation
KW  - cytoskeleton
Y1  - 2014
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-118406
VL  - 9
IS  - 5
ER  - 
TY  - JOUR
A1  - Dusik, Verena
A1  - Senthilan, Pingkalai R.
A1  - Mentzel, Benjamin
A1  - Hartlieb, Heiko
A1  - Wülbeck, Corina
A1  - Yoshii, Taishi
A1  - Raabe, Thomas
A1  - Helfrich-Förster, Charlotte
T1  - The MAP Kinase p38 Is Part of Drosophila melanogaster's Circadian Clock
JF  - PLoS Genetics
N2  - All organisms have to adapt to acute as well as to regularly occurring changes in the environment. To deal with these major challenges organisms evolved two fundamental mechanisms: the p38 mitogen-activated protein kinase (MAPK) pathway, a major stress pathway for signaling stressful events, and circadian clocks to prepare for the daily environmental changes. Both systems respond sensitively to light. Recent studies in vertebrates and fungi indicate that p38 is involved in light-signaling to the circadian clock providing an interesting link between stress-induced and regularly rhythmic adaptations of animals to the environment, but the molecular and cellular mechanisms remained largely unknown. Here, we demonstrate by immunocytochemical means that p38 is expressed in Drosophila melanogaster's clock neurons and that it is activated in a clock-dependent manner. Surprisingly, we found that p38 is most active under darkness and, besides its circadian activation, additionally gets inactivated by light. Moreover, locomotor activity recordings revealed that p38 is essential for a wild-type timing of evening activity and for maintaining ∼ 24 h behavioral rhythms under constant darkness: flies with reduced p38 activity in clock neurons, delayed evening activity and lengthened the period of their free-running rhythms. Furthermore, nuclear translocation of the clock protein Period was significantly delayed on the expression of a dominant-negative form of p38b in Drosophila's most important clock neurons. Western Blots revealed that p38 affects the phosphorylation degree of Period, what is likely the reason for its effects on nuclear entry of Period. In vitro kinase assays confirmed our Western Blot results and point to p38 as a potential "clock kinase" phosphorylating Period. Taken together, our findings indicate that the p38 MAP Kinase is an integral component of the core circadian clock of Drosophila in addition to playing a role in stress-input pathways.
KW  - in vitro kinase assay
KW  - biological locomotion
KW  - circadian oscillators
KW  - MAPK signaling cascades
KW  - circadian rhythms
KW  - drosophila melanogaster
KW  - neurons
KW  - phosphorylation
Y1  - 2014
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-119433
SN  - 1553-7404
VL  - 10
IS  - 8
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  - JOUR
A1  - Röder, Pia V.
A1  - Geillinger, Kerstin E.
A1  - Zietek, Tamara S.
A1  - Thorens, Bernard
A1  - Koepsell, Hermann
A1  - Daniel, Hannelore
T1  - The Role of SGLT1 and GLUT2 in Intestinal Glucose Transport and Sensing
JF  - PLOS ONE
N2  - Intestinal glucose absorption is mediated by SGLT1 whereas GLUT2 is considered to provide basolateral exit. Recently, it was proposed that GLUT2 can be recruited into the apical membrane after a high luminal glucose bolus allowing bulk absorption of glucose by facilitated diffusion. Moreover, SGLT1 and GLUT2 are suggested to play an important role in intestinal glucose sensing and incretin secretion. In mice that lack either SGLT1 or GLUT2 we re-assessed the role of these transporters in intestinal glucose uptake after radiotracer glucose gavage and performed Western blot analysis for transporter abundance in apical membrane fractions in a comparative approach. Moreover, we examined the contribution of these transporters to glucose-induced changes in plasma GIP, GLP-1 and insulin levels. In mice lacking SGLT1, tissue retention of tracer glucose was drastically reduced throughout the entire small intestine whereas GLUT2-deficient animals exhibited higher tracer contents in tissue samples than wild type animals. Deletion of SGLT1 resulted also in reduced blood glucose elevations and abolished GIP and GLP-1 secretion in response to glucose. In mice lacking GLUT2, glucose-induced insulin but not incretin secretion was impaired. Western blot analysis revealed unchanged protein levels of SGLT1 after glucose gavage. GLUT2 detected in apical membrane fractions mainly resulted from contamination with basolateral membranes but did not change in density after glucose administration. SGLT1 is unequivocally the prime intestinal glucose transporter even at high luminal glucose concentrations. Moreover, SGLT1 mediates glucose-induced incretin secretion. Our studies do not provide evidence for GLUT2 playing any role in either apical glucose influx or incretin secretion.
KW  - rat small-intestine
KW  - brush border membrane
KW  - apical GLUT2
KW  - incretin secretion
KW  - diffusive component
KW  - sugar absorption
KW  - mice
KW  - calcium absorption
KW  - phosphorylation
KW  - cotransporter
Y1  - 2014
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-117262
VL  - 9
IS  - 2
ER  -