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Start Over Author "Schroeder V" Journal molecular immunology
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4. Role of complement in diabetes.

Author

Ajjan RA and Schroeder V

Subjects
Animals, Humans, Insulin Resistance immunology, Vascular Diseases immunology, Complement System Proteins immunology, Diabetes Mellitus, Type 1 immunology, Diabetes Mellitus, Type 2 immunology
Abstract

Accumulating evidence suggests a role for the complement system in the pathogenesis of diabetes and the vascular complications that characterise this condition. Complement proteins contribute to the development of type 1 diabetes (T1D) by enhancing the underlying organ-specific autoimmune processes. Complement upregulation and activation is also an important feature of insulin resistance and the development of type 2 diabetes (T2D). Moreover, animal and human studies indicate that complement proteins are involved in the pathogenic mechanisms leading to diabetic microvascular and macrovascular complications. The adverse vascular effects of complement appear to be related to enhancement of the inflammatory process and the predisposition to a thrombotic environment, eventually leading to vascular occlusion. Complement proteins have been considered as therapeutic targets to prevent or treat vascular disease but studies have been mainly conducted in animal models, while human work has been both limited and inconclusive so far. Further studies are needed to understand the potential role of complement proteins as therapeutic targets for reversal of the pathological processes leading to T1D and T2D and for the prevention/treatment of diabetic vascular complications., (Copyright © 2019 Elsevier Ltd. All rights reserved.)

Published
2019
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5. MASP-1 of the complement system alters fibrinolytic behaviour of blood clots.

Author

Jenny L, Noser D, Larsen JB, Dobó J, Gál P, Pál G, and Schroeder V

Subjects
Humans, Plasma immunology, Plasminogen immunology, Blood Coagulation immunology, Complement System Proteins immunology, Fibrin immunology, Fibrinolysis immunology, Mannose-Binding Protein-Associated Serine Proteases immunology, Thrombosis immunology
Abstract

Background: The lectin pathway serine protease mannan-binding lectin-associated serine protease 1 (MASP-1) has been demonstrated to be a major link between complement and coagulation, yet little is known about its interactions with the fibrinolytic system. The aim of this work was to assess the effects of MASP-1 on fibrin clot lysis in different experimental settings., Methods: Rotational thrombelastometry was used to evaluate the effect of MASP-1 on the lysis of clots formed in whole blood under static conditions. Whole blood clots were also formed in the presence and absence of MASP-1 under flow conditions in the Chandler loop and their lysis was analysed separately by fluorescence release of incorporated labelled fibrin. Real-time observation by laser scanning confocal microscopy was used to investigate the lysis of plasma clots where MASP-1 was present either during clot formation or lysis. Cleavage of tPA or plasminogen by MASP-1 was analysed by gel electrophoresis. We performed a turbidimetric clot lysis assay in the presence and absence of the MASP-1 inhibitor SGMI-1 (Schistocerca gregaria protease inhibitor (SGPI)-based MASP inhibitor-1) to evaluate the effect of endogenous MASP-1 in normal plasma and plasma samples from sepsis patients., Results: In the thrombelastometric experiments, where MASP-1 was present during the entire clotting and lysis process, MASP-1 had a significant profibrinolytic effect and accelerated clot lysis. When clots were formed in the presence of MASP-1 under flow in the Chandler loop, the effects on fibrinolysis were heterogenous with impaired fibrinolysis in some individuals (n = 5) and no (n = 3) or even the opposite effect (n = 2) in others. In plasma clot lysis observed by confocal microscopy, lysis was prolonged when MASP-1 was added to the lysis solution, yet there was no difference in lysis time when MASP-1 was present during clot formation. When MASP-1 was incubated with tPA or plasminogen, respectively, cleavage of single-chain tPA into two-chain tPA and a slight reduction of plasminogen were observed. SGMI-1 significantly prolonged clot lysis in the turbidimetric clot lysis assay suggesting that MASP-1 accelerated lysis in plasma samples., Conclusion: MASP-1 is able to alter the susceptibility of blood clots to the fibrinolytic system. MASP-1 has complex, mostly promoting effects on fibrinolysis with high inter-individual variation. Interactions of MASP-1 with the fibrinolytic system may be relevant in the development and therapy of cardiovascular and thrombotic diseases., (Copyright © 2019 Elsevier Ltd. All rights reserved.)

Published
2019
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6. MASP-1 of the complement system promotes clotting via prothrombin activation.

Author

Jenny L, Dobó J, Gál P, and Schroeder V

Subjects
Enzyme Activation immunology, Female, Humans, Male, Mannose-Binding Protein-Associated Serine Proteases immunology, Prothrombin immunology, Thrombelastography, Blood Coagulation, Mannose-Binding Protein-Associated Serine Proteases chemistry, Proteolysis, Prothrombin chemistry
Abstract

Mannan-binding lectin-associated serine protease-1 (MASP-1), a protein of the complement lectin pathway, resembles thrombin in terms of structural features and substrate specificity, and it has been shown to activate coagulation factors. Here we studied the effects of MASP-1 on clot formation in whole blood (WB) and platelet-poor plasma (PPP) by thrombelastography and further elucidated the underlying mechanism. Cleavage of prothrombin by MASP-1 was investigated by SDS-PAGE and N-terminal sequencing of cleavage products. Addition of MASP-1 or thrombin to WB and PPP shortened the clotting time and clot formation time significantly compared to recalcified-only samples. The combination of MASP-1 and thrombin had additive effects. In a purified system, MASP-1 was able to induce clotting only in presence of prothrombin. Analysis of MASP-1-digested prothrombin confirmed that MASP-1 cleaves prothrombin at three cleavage sites. In conclusion, we have shown that MASP-1 is able to induce and promote clot formation measured in a global setting using the technique of thrombelastography. We further confirmed that MASP-1-induced clotting is dependent on prothrombin. Finally, we have demonstrated that MASP-1 cleaves prothrombin and identified its cleavage sites, suggesting that MASP-1 gives rise to an alternative active form of thrombin by cleaving at the cleavage site R393., (Copyright © 2015 Elsevier Ltd. All rights reserved.)

Published
2015
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7. Multiple roles of complement MASP-1 at the interface of innate immune response and coagulation.

Author

Dobó J, Schroeder V, Jenny L, Cervenak L, Závodszky P, and Gál P

Subjects
Animals, Blood Coagulation Factors metabolism, Complement Pathway, Mannose-Binding Lectin physiology, Humans, Mannose-Binding Protein-Associated Serine Proteases chemistry, Protein Binding, Blood Coagulation physiology, Immunity, Innate physiology, Mannose-Binding Protein-Associated Serine Proteases metabolism
Abstract

MASP-1 is a versatile serine protease that cleaves a number of substrates in human blood. In recent years it became evident that besides playing a crucial role in complement activation MASP-1 also triggers other cascade systems and even cells to mount a more powerful innate immune response. In this review we summarize the latest discoveries about the diverse functions of this multi-faceted protease. Recent studies revealed that among MBL-associated serine proteases, MASP-1 is the one responsible for triggering the lectin pathway via its ability to rapidly autoactivate then cleave MASP-2, and possibly MASP-3. The crystal structure of MASP-1 explains its more relaxed substrate specificity compared to the related complement enzymes. Due to the relaxed specificity, MASP-1 interacts with the coagulation cascade and the kinin generating system, and it can also activate endothelial cells eliciting pro-inflammatory signaling., (Copyright © 2014 Elsevier Ltd. All rights reserved.)

Published
2014
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