The Gp1ba-Cre transgenic mouse::A new model to delineate platelet and leukocyte functions

Conditional knockout (KO) mouse models are invaluable for elucidating the physiological roles of platelets. The Platelet factor 4-Cre recombinase (Pf4-Cre) transgenic mouse is the current model of choice for generating megakaryocyte/platelet-specific KO mice. Platelets and leukocytes work closely together in a wide range of disease settings, yet the specific contribution of platelets to these processes remains unclear. This is partially a result of the Pf4-Cre transgene being expressed in a variety of leukocyte populations. To overcome this issue, we developed a Gp1ba-Cre transgenic mouse strain in which Cre expression is driven by the endogenous Gp1ba locus. By crossing Gp1ba-Cre and Pf4-Cre mice to the mT/mG dual-fluorescence reporter mouse and performing a head-to-head comparison, we demonstrate more stringent megakaryocyte lineage-specific expression of the Gp1ba-Cre transgene. Broader tissue expression was observed with the Pf4-Cre transgene, leading to recombination in many hematopoietic lineages, including monocytes, macrophages, granulocytes, and dendritic and B and T cells. Direct comparison of phenotypes of Csk, Shp1, or CD148 conditional KO mice generated using either the Gp1ba-Cre or Pf4-Cre strains revealed similar platelet phenotypes. However, additional inflammatory and immunological anomalies were observed in Pf4-Cre-generated KO mice as a result of nonspecific deletion in other hematopoietic lineages. By excluding leukocyte contributions to phenotypes, the Gp1ba-Cre mouse will advance our understanding of the role of platelets in inflammation and other pathophysiological processes in which platelet-leukocyte interactions are involved

Loss of zinc transporters ZIP1 and ZIP3 augments platelet reactivity in response to thrombin and accelerates thrombus formation in vivo

Zinc (Zn2+) is considered as important mediator of immune cell function, thrombosis and haemostasis. However, our understanding of the transport mechanisms that regulate Zn2+ homeostasis in platelets is limited. Zn2+ transporters, ZIPs and ZnTs, are widely expressed in eukaryotic cells. Using mice globally lacking ZIP1 and ZIP3 (ZIP1/3 DKO), our aim was to explore the potential role of these Zn2+ transporters in maintaining platelet Zn2+ homeostasis and in the regulation of platelet function. While ICP-MS measurements indicated unaltered overall Zn2+ concentrations in platelets of ZIP1/3 DKO mice, we observed a significantly increased content of FluoZin3-stainable free Zn2+, which, however, appears to be released less efficiently upon thrombin-stimulated platelet activation. On the functional level, ZIP1/3 DKO platelets exhibited a hyperactive response towards threshold concentrations of G protein-coupled receptor (GPCR) agonists, while immunoreceptor tyrosine-based activation motif (ITAM)-coupled receptor agonist signalling was unaffected. This resulted in enhanced platelet aggregation towards thrombin, bigger thrombus volume under flow ex vivo and faster in vivo thrombus formation in ZIP1/3 DKO mice. Molecularly, augmented GPCR responses were accompanied by enhanced Ca2+ and PKC, CamKII and ERK1/2 signalling. The current study thereby identifies ZIP1 and ZIP3 as important regulators for the maintenance of platelet Zn2+ homeostasis and function

Studien zur Signaltransduktion und Regulierung von Rezeptoren in Thrombozyten und T-Zellen genetisch veränderter Mäuse

Receptors with tyrosine-based signaling motifs control essential functions of hematopoietic cells, including lymphocytes and platelets. Downstream of the platelet receptor glycoprotein (GP) VI and the T cell receptor (TCR) the immunoreceptor tyrosine-based activation motif (ITAM) initiates a signaling cascade that involves kinases, adapter and effector proteins and finally leads to cellular activation. This thesis summarizes the results of three studies investigating different aspects of receptor signaling and regulation in platelets and T cells. In the first part, the impact of constitutive Ca2+ influx on TCR signaling and T cell physiology was investigated using a transgenic mouse line with a mutation in the Ca2+ sensor stromal interaction molecule 1 (STIM1). The elevated cytoplasmic Ca2+ level resulted in an altered phosphorylation pattern of the key enzyme phospholipase (PL) Cγ1 in response to TCR stimulation, but without affecting its enzymatic activity. Withdrawal of extracellular Ca2+ or inhibition of the phosphatase calcineurin restored the normal phosphorylation pattern. In addition, there was a decrease in the release of Th2-type cytokines interleukin 4, 5 and 13 upon stimulation in vitro. The second part of the thesis deals with the role of the adapter protein growth factor receptor-bound protein 2 (Grb2) in platelets using a megakaryocyte/platelet-specific knockout mouse line. Loss of Grb2 severely impaired signaling of GPVI and C-type lectin-like receptor 2 (CLEC-2), a related hemITAM receptor. This was attributed to defective stabilization of the linker for activation of T cells (LAT) signalosome and resulted in reduced adhesion, aggregation, Ca2+ mobilization and procoagulant activity downstream of (hem)ITAM-coupled receptors in vitro. In contrast, the signaling pathways of G protein-coupled receptors (GPCRs) and the integrin αIIbβ3, which do not utilize the LAT signalosome, were unaffected. In vivo, the defective (hem)ITAM signaling caused prolonged bleeding times, however, thrombus formation was only affected under conditions where GPCR signaling was impaired (upon acetylsalicylic acid treatment). These results establish Grb2 as an important adapter protein in the propagation of GPVI- and CLEC-2-induced signals. Finally, the proteolytic regulation of the immunoreceptor tyrosine-based switch motif (ITSM)-bearing receptor CD84 in platelets was investigated. This study demonstrated that in mice CD84 is cleaved by two distinct and independent proteolytic mechanisms upon platelet activation: shedding of the extracellular part, which is exclusively mediated by a disintegrin and metalloproteinase (ADAM) 10 and cleavage of the intracellular C-terminus by the protease calpain. Finally, the analysis of soluble CD84 levels in the plasma of transgenic mice revealed that shedding of CD84 by ADAM10 occurs constitutively in vivo.Rezeptoren mit Tyrosin-basierten Signaltransduktionsmotiven sind von fundamentaler Bedeutung für die Funktion hematopoietischer Zellen wie Lymphozyten und Thrombozyten. Unterhalb des Glykoproteins (GP) VI auf Thrombozyten und des T-Zell Rezeptors (TZR) auf T-Zellen initiiert das immunoreceptor tyrosine-based activation motif (ITAM) eine Signalkaskade, die Kinasen, Adapter- und Effektorproteine mit einbezieht und schlussendlich zur Aktivierung der Zelle führt. Die hier vorgelegte Arbeit fasst die Ergebnisse dreier Studien zusammen, die sich mit verschiedenen Aspekten der Signaltransduktion und Regulation von Rezeptoren in Thrombozyten und T-Zellen befasst. Im ersten Teil wurde der Einfluss eines konstitutiven Ca2+-Einstroms auf die TZR Signalkaskade und T-Zell Funktion untersucht. Hierzu wurde eine transgene Mauslinie mit einer Mutation im Ca2+-Sensor stromal interaction molecule 1 (STIM1) verwendet. Die erhöhte zytoplasmatische Ca2+-Konzentration veränderte das Phosphorylierungsmuster der Phospholipase (PL) Cγ1, ein Schlüsselenzym der Signalkaskade, nach Stimulation des TZRs. Die enzymatische Aktivität der PLCγ1 blieb hierbei jedoch unverändert. In der Abwesenheit von extrazellulärem Ca2+ oder bei Inhibition der Phosphatase Calcineurin war das Phosphorylierungsmuster hingegen wieder normal. Darüber hinaus zeigten die T Zellen nach Stimulation in vitro eine verringerte Produktion von Interleukinen des Th2-Typs (Interleukin-4, 5 und 13). Der zweite Teil der Arbeit befasst sich mit der Funktion des Adapterproteins growth factor receptor-bound protein 2 (Grb2) in Thrombozyten, die unter Zuhilfenahme einer Megakaryozyten- und Thrombozyten-spezifischen Knockout Mauslinie untersucht wurde. Hierbei zeigte es sich, dass der Verlust von Grb2 die Signaltransduktion von GPVI und des verwandten hemITAM-Rezeptors C type lectin-like receptor 2 (CLEC-2) schwer beeinträchtigt. Dies konnte auf eine mangelnde Stabilisierung des linker for activation of T cells (LAT) Signalosoms zurückgeführt werden und resultierte in einer verminderten Adhäsion, Aggregation, Ca2+-Mobilisierung und prokoagulatorischen Aktivität nach Aktivierung (hem)ITAM gekoppelter Rezeptoren in vitro. Im Gegensatz hierzu blieben die Signaltransduktionswege G-protein-gekoppelter Rezeptoren (GPCRs) und des Integrins αIIbβ3, die das LAT Signalosom nicht nutzen, unbeeinflusst. In in vivo Studien verursachte die beeinträchtigte (hem)ITAM Signaltransduktion eine verlängerte Blutungszeit der Mäuse, während die Entstehung von Thromben nur bei gleichzeitiger Hemmung von GPCR-Signalwegen (durch Acetylsalicylsäuregabe) vermindert war. Diese Ergebnisse etablieren Grb2 als ein wichtiges Adapterprotein in der Signaltransduktionskaskade von GPVI und CLEC-2. Schließlich wurde im dritten Teil dieser Arbeit die proteolytische Regulation des Rezeptors CD84, der ein immunoreceptor tyrosine-based switch motif (ITSM) enthält, untersucht. In dieser Studie konnte gezeigt werden, dass CD84 in Mausthrombozyten durch zwei verschiedene und unabhängige proteolytische Mechanismen geschnitten wird: Zum einen durch Shedding des extrazellulären Teils, was ausschließlich durch die a disintegrin and metalloproteinase (ADAM) 10 bewerkstelligt wird, und zum anderen durch das Schneiden des intrazellulären C Terminus durch die Protease Calpain. Des Weiteren zeigte eine Untersuchung von Plasmaproben transgener Mäuse, dass das Shedding von CD84 durch ADAM10 konstitutiv in vivo erfolgt

Mice lacking the SLAM family member CD84 display unaltered platelet function in hemostasis and thrombosis

Background Platelets are anuclear cell fragments derived from bone marrow megakaryocytes that safeguard vascular integrity by forming thrombi at sites of vascular injury. Although the early events of thrombus formation—platelet adhesion and aggregation—have been intensively studied, less is known about the mechanisms and receptors that stabilize platelet-platelet interactions once a thrombus has formed. One receptor that has been implicated in this process is the signaling lymphocyte activation molecule (SLAM) family member CD84, which can undergo homophilic interactions and becomes phosphorylated upon platelet aggregation. Objective The role of CD84 in platelet physiology and thrombus formation was investigated in CD84-deficient mice. Methods and Results We generated CD84-deficient mice and analyzed their platelets in vitro and in vivo. $Cd84^{−/−}$ platelets exhibited normal activation and aggregation responses to classical platelet agonists. Furthermore, CD84 deficiency did not affect integrin-mediated clot retraction and spreading of activated platelets on fibrinogen. Notably, also the formation of stable three-dimensional thrombi on collagen-coated surfaces under flow ex vivo was unaltered in the blood of $Cd84^{−/−}$ mice. In vivo, $Cd84^{−/−}$ mice exhibited unaltered hemostatic function and arterial thrombus formation. Conclusion These results show that CD84 is dispensable for thrombus formation and stabilization, indicating that its deficiency may be functionally compensated by other receptors or that it may be important for platelet functions different from platelet-platelet interactions

CD84-deficient mice display normal platelet count and size.

<p>(A) CD84 targeting strategy: This scheme illustrates the detection of wild-type and <i>Cd84^−/−</i> (targeted) alleles. Upon homologous recombination, the pWH9 cassette containing a neomycin resistance gene disrupts the <i>Cd84</i> gene. An external probe (EP) recognizes a sequence downstream of 3′ arm in intron 2. With the pWH9 cassette, a new <i>Bam</i>HI restriction site is introduced, enabling the determination of a wild-type and <i>Cd84^−/−</i> band by Southern blot analysis. (B) Analysis of CD84 expression in wild-type (<i>Cd84^+/+</i>) and <i>Cd84^−/−</i> platelets by Western blot. Expression of GPIIIa was used as loading control. (C) Peripheral platelet counts and (D) platelet volume of wild-type and <i>Cd84^−/−</i> mice measured with a blood cell counter. (E) Determination of the platelet life span in wild-type and <i>Cd84^−/−</i> mice. Mice were injected with a DyLight 488-conjugated anti-GPIX Ig derivate to label platelets <i>in vivo</i>. Results are % of fluorescently labeled platelets at the indicated days after injection as determined by flow cytometry. Values are mean ± SD of 5 mice per group.</p

<i>Cd84⁻</i>^/<i>−</i> mice display normal hematologic parameters and unaltered levels of platelet surface glycoproteins.

<p>(A) White blood cell (WBC) count, red blood cell (RBC) count, hemoglobin (HGB) and hematocrit (HCT) were determined with a hematologic analyzer (Sysmex) (n = 5, two independent experiments, n.s.  =  not significant). (B) Expression of glycoproteins on the platelet surface was determined by flow cytometry. Diluted whole blood from the indicated mice was incubated with FITC-labeled antibodies at saturating conditions for 15 minutes at RT, and platelets were analyzed directly. Data are expressed as mean fluorescence intensity ± SD (n = 4) and are representative of 3 individual experiments.</p><p><i>Cd84⁻</i>^/<i>−</i> mice display normal hematologic parameters and unaltered levels of platelet surface glycoproteins.</p

Critical redundant functions of the adapters Grb2 and Gads in platelet (hem)ITAM signaling in mice

Platelets are essential for normal hemostasis; however, pathological conditions can also trigger unwanted platelet activation precipitating thrombosis and ischemic damage of vital organs such as the heart or brain. Glycoprotein (GP)VI- and C-type lectin-like receptor 2 (CLEC-2)-mediated (hem)immunoreceptor tyrosine-based activation motif (ITAM) signaling represents a major pathway for platelet activation. The two members of the Growth-factor receptor-bound protein 2 (Grb2) family of adapter proteins expressed in platelets – Grb2 and Grb2-related adapter protein downstream of Shc (Gads) – are part of the hem(ITAM) signaling cascade by forming an adapter protein complex with linker for activation of T cells (LAT). To date, a possible functional redundancy between these two adapters in platelet activation has not been investigated. We here generated megakaryocyte- and platelet-specific Grb2/Gads double knockout (DKO) mice and analyzed their platelet function in vitro and in vivo. The DKO platelets exhibited virtually abolished (hem)ITAM signaling whereas only partial defects were seen in Grb2 or Gads single-deficient platelets. This was based on impaired phosphorylation of key molecules in the (hem)ITAM signaling cascade and translated into impaired hemostasis and partially defective arterial thrombosis, thereby exceeding the defects in either Grb2 KO or Gads KO mice. Despite this severe (hem)ITAM signaling defect, CLEC-2 dependent regulation of blood-lymphatic vessel separation was not affected in the DKO animals. These results provide direct evidence for critically redundant roles of Grb2 and Gads for platelet function in hemostasis and thrombosis, but not development

Targeted downregulation of platelet CLEC-2 occurs through Syk-independent internalization

Platelet aggregation at sites of vascular injury is not only essential for hemostasis, but may also cause acute ischemic disease states such as myocardial infarction or stroke. The hemi-immunoreceptor tyrosine-based activation motif–containing C-type lectinlike receptor 2 (CLEC-2) mediates powerful platelet activation through a Src- and spleen tyrosine kinase (Syk)–dependent tyrosine phosphorylation cascade. Thereby, CLEC-2 not only contributes to thrombus formation and stabilization but also plays a central role in blood-lymphatic vessel development, tumor metastasis, and prevention of inflammatory bleeding, making it a potential pharmacologic target to modulate these processes. We have previously shown that injection of the anti–CLEC-2 antibody, INU1, results in virtually complete immunodepletion of platelet CLEC-2 in mice, which is, however, preceded by a severe transient thrombocytopenia thereby limiting its potential therapeutic use. The mechanisms underlying this targeted CLEC-2 downregulation have remained elusive. Here, we show that INU1-induced CLEC-2 immunodepletion occurs through Src-family kinase–dependent receptor internalization in vitro and in vivo, presumably followed by intracellular degradation. In mice with platelet-specific Syk deficiency, INU1-induced CLEC-2 internalization/degradation was fully preserved whereas the associated thrombocytopenia was largely prevented. These results show for the first time that CLEC-2 can be downregulated from the platelet surface through internalization in vitro and in vivo and that this can be mechanistically uncoupled from the associated antibody-induced thrombocytopenia

Growth factor receptor-bound protein 2 contributes to (hem)immunoreceptor tyrosine-based activation motif-mediated signaling in platelets

Rationale: Platelets are anuclear cell fragments derived from bone marrow megakaryocytes (MKs) that safeguard vascular integrity but may also cause pathological vessel occlusion. One major pathway of platelet activation is triggered by 2 receptors that signal through an (hem)immunoreceptor tyrosine-based activation motif (ITAM), the activating collagen receptor glycoprotein (GP) VI and the C-type lectin-like receptor 2 (CLEC-2). Growth factor receptor–bound protein 2 (Grb2) is a ubiquitously expressed adapter molecule involved in signaling processes of numerous receptors in different cell types, but its function in platelets and MKs is unknown. Objective: We tested the hypothesis that Grb2 is a crucial adapter protein in (hem)immunoreceptor tyrosine-based activation motif signaling in platelets. Methods and Results: Here, we show that genetic ablation of Grb2 in MKs and platelets did not interfere with MK differentiation or platelet production. However, Grb2-deficiency severely impaired glycoprotein VI–mediated platelet activation because of defective stabilization of the linker of activated T-cell (LAT) signalosome and activation of downstream signaling proteins that resulted in reduced adhesion, aggregation, and coagulant activity on collagen in vitro. Similarly, CLEC-2–mediated signaling was impaired in Grb2-deficient platelets, whereas the cells responded normally to stimulation of G protein–coupled receptors. In vivo, this selective (hem)immunoreceptor tyrosine-based activation motif signaling defect resulted in prolonged bleeding times but affected arterial thrombus formation only after concomitant treatment with acetylsalicylic acid, indicating that defective glycoprotein VI signaling in the absence of Grb2 can be compensated through thromboxane A2–induced G protein–coupled receptor signaling pathways. Conclusions: These results reveal an important contribution of Grb2 in (hem)immunoreceptor tyrosine-based activation motif signaling in platelets in hemostasis and thrombosis by stabilizing the LAT signalosome