Your search keyword '"Muchitsch EM"' showing total 37 results

1. 'Protective effect of Human-Derived Protein C in Septic Neonatal Mice.'

Author

MUCHITSCH EM, SCHWARZ HP, VRADI K, ESMON C, TETI G., MANCUSO, Giacomo, MUCHITSCH EM, SCHWARZ HP, VRADI K, ESMON C, MANCUSO G, and TETI G

Published

2005

2. Human plasma-derived protein C and murine recombinant protein C: Effect on severe neonatal sepsis in mice

Author

Muchitsch, Em, Schwarz, Hp, Varadi, K, Esmon, C, Mancuso, Giuseppe, and Teti, Giuseppe

Published

2005

3. Effects of alpha 1-acid glycoprotein in different rodent models of shock

Author

Muchitsch Em, W. Auer, and Pichler L

Subjects

Lipopolysaccharides, Male, Salmonella typhimurium, Resuscitation, Alpha (ethology), Orosomucoid, Pharmacology, Peritonitis, Shock, Hemorrhagic, Sepsis, Rats, Sprague-Dawley, Mice, Species Specificity, Hypovolemia, medicine, Animals, Humans, Pharmacology (medical), biology, business.industry, Acute-phase protein, Hemodynamics, medicine.disease, Survival Analysis, Rats, Mice, Inbred C57BL, Disease Models, Animal, Shock (circulatory), Immunology, biology.protein, Female, medicine.symptom, business, Perfusion

Abstract

It was the aim of the present study to investigate the effects of the acute phase protein alpha 1-acid glycoprotein in different models of shock. The human plasma preparation used was without effect on mortality in lipopolysaccharide-injected mice when administered in two different doses (1 or 0.33 g/kg i.v.) and according to different treatment schedules. The same preparation significantly increased survival rate (48 h) in rats with septic peritonitis. This effect was seen when alpha 1-acid glycoprotein (200 mg/kg i.v.) was given 15 min prior to and 24 h after cecal puncture. All other dose regimes tested were without significant effect on survival rate. A hemorrhagic/hypovolemic shock model (including a defined trauma) in rats resuscitated with 200 mg/kg alpha 1-acid glycoprotein resulted in significantly higher values of mean arterial blood pressure, cardiac output and stroke volume when compared to corresponding values obtained after resuscitation with Ringer's solution or 200 mg/kg albumin i.v. (free of alpha 1-acid glycoprotein; placebo formulation). Taking all other possible mechanisms of alpha 1-acid glycoprotein into consideration, the partially protective effects of the preparation are explained by enhancing the capillary barrier function and thereby maintaining perfusion of vital organs.

Published

1998

4. Liver expression of hepcidin and other iron genes in two mouse models of beta-thalassemia

Author

Lucia, De Franceschi, Filomena, Daraio, Alida, Filippini, Sonia, Carturan, Eva Maria, Muchitsch, Antonella, Roetto, Clara, Camaschella, DE FRANCESCHI, L, Daraio, F, Filippini, A, Carturan, S, Muchitsch, Em, Roetto, A, and Camaschella, Clara

Subjects

Mice, Knockout, thalassemia, Iron Overload, Iron, beta-Thalassemia, anemia, Mice, Mutant Strains, Mice, Inbred C57BL, Disease Models, Animal, Mice, Gene Expression Regulation, Hepcidins, Liver, Mice, Inbred DBA, iron metabolism, hepcidin, Animals, Female, Antimicrobial Cationic Peptides

Abstract

Homozygous beta-thalassemia patients may develop iron overload even if untransfused, due to inappropriately high intestinal iron absorption. Reduction of hepcidin synthesis has been reported both in patients and in animal models. We have measured liver hepcidin and other iron gene transcripts in two different mouse models of beta-thalassemia at different ages.Mice Hbb(th/th), characterized by spontaneous homozygous deletion of the major b1 globin gene were studied at 2 and 8 months. Mice Hbb(th/3+), characterized by the heterozygous deletion of b1 and b2 globin genes were studied at 4 and 10 months. Hematologic data were obtained and iron overload estimated by Perls' staining of the liver. Expression of liver hepcidin, Tfr2, Hjv, Fpn and Hfe RNA was assessed by real-time polymerase chain reaction. Levels of serum cytokines (interleukin-6, IL-1beta, IL-10, granulocyte-macrophage colony-stimulating factor) levels were assayed by enzyme-linked immunosorbent assay.Hemoglobin, hematocrit and mean corpuscular volume were significantly reduced in both beta-thalassemia models, more significantly in Hbb(th/3+), which have the greater, age-dependent, iron overload. Hepcidin RNA was not increased despite iron overload in both strains. Fpn RNA was increased and Tfr2 was decreased in older animals. Inflammatory cytokine levels were striking variable and unrelated to hepcidin levels.Although anemia is reported to inhibit hepcidin expression, normal hepcidin synthesis was maintained in both thalassemic models studied. However, hepcidin levels were inappropriate for the body iron, especially in Hbb(th/3+) 10-month-old animals. As we previously reported in wild type mice after parenteral iron overload, Tfr2 is reduced and Fpn RNA increased in thalassemic mice. Inflammatory cytokines did not play a major role in increasing hepcidin levels or in modifying iron homeostasis in this study.

Published

2006

5. Pharmacokinetics, disease-modifying activity, and safety of an experimental therapeutic targeting an immunological isoform of macrophage migration inhibitory factor, in rat glomerulonephritis.

Author

Höllriegl W, Bauer A, Baumgartner B, Dietrich B, Douillard P, Kerschbaumer RJ, Höbarth G, McKee JS, Schinagl A, Tam FWK, Thiele M, Weber A, Wolfsegger M, Turecek M, Muchitsch EM, Scheiflinger F, and Glantschnig H

Subjects

Animals, Antibodies, Monoclonal adverse effects, Antibodies, Monoclonal immunology, Cell Movement drug effects, Cell Proliferation drug effects, Disease Progression, Female, Glomerulonephritis metabolism, Humans, Kidney Glomerulus drug effects, Kidney Glomerulus pathology, Male, Monocytes cytology, Monocytes drug effects, Protein Isoforms immunology, Rats, Antibodies, Monoclonal pharmacokinetics, Antibodies, Monoclonal therapeutic use, Glomerulonephritis drug therapy, Glomerulonephritis immunology, Macrophage Migration-Inhibitory Factors immunology, Molecular Targeted Therapy, Safety

Abstract

New therapeutic agents are needed to overcome the toxicity and suboptimal efficacy observed in current treatment of glomerulonephritis (GN). BaxB01 is a fully human monoclonal antibody targeting a disease-related immunologically distinct isoform of Macrophage migration Inhibitory Factor (MIF), designated oxidized MIF (oxMIF) and locally expressed in inflammatory conditions. We report the pharmacokinetic profile of BaxB01, and its dose and exposure-related disease-modifying activity in experimentally induced rat GN. BaxB01 bound to rat oxMIF with high affinity and reduced rat macrophage migration in vitro. After intravenous administration in rats, BaxB01 demonstrated favorable pharmacokinetics, with a half-life of up to nine days. Disease modification was dose-related (≥ 10mg/kg) as demonstrated by significantly reduced proteinuria and diminished histopathological glomerular crescent formation. Importantly, a single dose was sufficient to establish an exposure-related, anti-inflammatory milieu via amelioration of glomerular cellular inflammation. Pharmacodynamic modeling corroborated these findings, consistently predicting plasma exposures that were effective in attenuating both anti-inflammatory activity and reducing loss of kidney function. This pharmacologic benefit on glomerular function and structure was sustained during established disease, while correlation analyses confirmed a link between the antibody's anti-inflammatory activity and reduced crescent formation in individual rats. Finally, safety assessment in rats showed that the experimental therapeutic was well tolerated without signs of systemic toxicity or negative impact on kidney function. These data define therapeutically relevant exposures correlated with mechanism-based activity in GN, while toxicological evaluation suggests a large therapeutic index and provides evidence for achieving safe and effective exposure to a MIF isoform-directed therapeutic in nephritis-associated disease., (Copyright © 2017 Elsevier B.V. All rights reserved.)

Published

2018

6. Preclinical assessment of a new recombinant ADAMTS-13 drug product (BAX930) for the treatment of thrombotic thrombocytopenic purpura.

Author

Kopić A, Benamara K, Piskernik C, Plaimauer B, Horling F, Höbarth G, Ruthsatz T, Dietrich B, Muchitsch EM, Scheiflinger F, Turecek M, and Höllriegl W

Subjects

ADAMTS13 Protein genetics, Animals, Area Under Curve, Blood Platelets drug effects, Disease Models, Animal, Drug Evaluation, Preclinical, Female, Humans, Macaca fascicularis, Male, Mice, Plasma metabolism, Platelet Count, Purpura, Thrombotic Thrombocytopenic blood, Rabbits, Rats, Recombinant Proteins pharmacology, Species Specificity, Thrombosis blood, Treatment Outcome, ADAMTS13 Protein pharmacology, Purpura, Thrombotic Thrombocytopenic drug therapy

Abstract

Unlabelled: Essentials ADAMTS-13-deficiency is a cause of thrombotic thrombocytopenic purpura (TTP). Preclinical safety of recombinant human ADAMTS-13 (BAX930) was shown in animal models. Preclinical efficacy of BAX930 was shown in a mouse model of TTP. BAX930 showed advantageous efficacy over fresh frozen plasma, the current standard of care. Click to hear Dr Cataland and Prof. Lämmle present a seminar on Thrombotic Thrombocytopenic Purpura (TTP): new Insights in Pathogenesis and Treatment Modalities., Summary: Background Thrombotic thrombocytopenic purpura (TTP) is a rare blood disorder characterized by microthrombosis in small blood vessels of the body, resulting in a low platelet count. Baxalta has developed a new recombinant ADAMTS-13 (rADAMTS-13) product (BAX930) for on-demand and prophylactic treatment of patients with hereditary TTP (hTTP). Objectives To evaluate the pharmacokinetics, efficacy and safety of BAX930 in different species, by use of an extensive preclinical program. Methods The prophylactic and therapeutic efficacies of BAX930 were tested in a previously established TTP mouse model. Pharmacokinetics were evaluated after single intravenous bolus injection in mice and rats, and after repeated dosing in cynomolgus monkeys. Toxicity was assessed in rats and monkeys, safety pharmacology in monkeys, and local tolerance in rabbits. Results BAX930 was shown to be efficacious, as demonstrated by a stabilized platelet count in ADAMTS-13 knockout mice that were thrombocytopenic when treated. Prophylactic efficacy was dose-dependent and comparable with that achieved by treatment with fresh frozen plasma, the mainstay of hTTP treatment. Therapeutic efficacy was treatment interval-dependent. Safety pharmacology evaluation did not show any deleterious effects of BAX930 on cardiovascular and respiratory functions in monkeys. The compound's pharmacokinetics were similar and dose-proportional in mice, rats, and monkeys. BAX930 was well tolerated in rats, monkeys, and rabbits, even at the highest doses tested. Conclusions These results demonstrate that BAX930 has a favorable preclinical profile, and support the clinical development of rADAMTS-13 for the treatment of hTTP., (© 2016 International Society on Thrombosis and Haemostasis.)

Published

2016

7. Nonacog gamma, a novel recombinant factor IX with low factor IXa content for treatment and prophylaxis of bleeding episodes.

Author

Turecek PL, Abbühl B, Tangada SD, Chapman M, Gritsch H, Rottensteiner H, Schrenk G, Mitterer A, Dietrich B, Höllriegl W, Schiviz A, Horling F, Reipert BM, Muchitsch EM, Pavlova BG, and Scheiflinger F

Subjects

Adult, Animals, CHO Cells, Child, Cricetinae, Cricetulus, Humans, Recombinant Proteins therapeutic use, Factor IX therapeutic use, Hemophilia B drug therapy, Hemostatics therapeutic use

Abstract

Nonacog gamma is a new recombinant factor IX to treat factor IX deficiency. It is indicated for control of bleeding episodes, perioperative management and routine prophylaxis to prevent or reduce the frequency of bleeding episodes in adults and children with hemophilia B. Nonacog gamma was first approved in the USA in June 2013 under the trade name RIXUBIS followed by market approvals in Australia and the EU in 2014, and marketing authorization decision is pending in Japan. Nonacog gamma is derived from a recombinant Chinese hamster ovary cell line using a state of the art biotechnological manufacturing process. Recombinant factor IX is produced by Baxter's protein-free fermentation technology, which was first developed for ADVATE. The product is purified and formulated in the absence of any human or animal-derived protein. Nonacog gamma was characterized both in comprehensive in vitro and in vivo non-clinical studies as well as in an extensive clinical trial program.

Published

2015

8. The biological efficacy profile of BAX 855, a PEGylated recombinant factor VIII molecule.

Author

Valentino LA, Cong L, Enockson C, Song X, Scheiflinger F, Muchitsch EM, Turecek PL, and Hakobyan N

Subjects

Animals, Disease Models, Animal, Hemorrhage prevention & control, Humans, Mice, Recombinant Proteins administration & dosage, Factor VIII administration & dosage, Hemophilia A drug therapy

Abstract

Prophylaxis prevents joint and other bleeding episodes in patients with haemophilia A. Development of new factor concentrates with longer circulating half-lives may encourage patients to start, continue or resume prophylaxis. The aim of this study was to compare the pharmacodynamic effect of a PEGylated full-length recombinant factor VIII (rFVIII) concentrate with that of an unmodified rFVIII concentrate with respect to the duration of prophylactic efficacy in a murine model of haemophilic joint bleeding. Mice were pretreated with BAX 855 or unmodified rFVIII at specified times before right knee puncture to induce haemarthrosis; left knee joints served as controls. Joint bleeding was evaluated using a combination of visual and histological assessments. Administration of a single dose of unmodified rFVIII before joint puncture prevented haemarthrosis in mice up to 24 h, whereas pretreatment with BAX 855 protected the joint from bleeding up to 48 h. This pharmacodynamic study showed prolonged efficacy of BAX 855 compared to ADVATE in a haemophilia A mouse joint bleeding model. This finding supports the possibility of using BAX 855 to increase FVIII trough levels and/or extend the dosing interval in patients with haemophilia A on prophylaxis, which may potentially improve prophylactic efficacy and long-term adherence., (© 2014 John Wiley & Sons Ltd.)

Published

2015

9. Influence of genetic background on bleeding phenotype in the tail-tip bleeding model and recommendations for standardization: communication from the SSC of the ISTH.

Author

Schiviz A, Magirr D, Leidenmühler P, Schuster M, Muchitsch EM, and Höllriegl W

Subjects

Animals, Disease Models, Animal, Factor VIII genetics, Factor VIII metabolism, Female, Genotype, Hemophilia A blood, Male, Mice, Mice, Inbred BALB C, Mice, Inbred C57BL, Mice, Knockout, Models, Animal, Phenotype, Sex Factors, Species Specificity, Bleeding Time standards, Genetic Variation, Hemophilia A genetics, Hemorrhage genetics

Published

2014

10. Preclinical safety and efficacy of a new recombinant FIX drug product for treatment of hemophilia B.

Author

Dietrich B, Schiviz A, Hoellriegl W, Horling F, Benamara K, Rottensteiner H, Turecek PL, Schwarz HP, Scheiflinger F, and Muchitsch EM

Subjects

Animals, Bleeding Time, Blood Coagulation drug effects, Disease Models, Animal, Drug Evaluation, Preclinical, Factor IX administration & dosage, Factor IX adverse effects, Hemophilia B blood, Humans, Macaca, Male, Mice, Rabbits, Rats, Recombinant Proteins administration & dosage, Recombinant Proteins adverse effects, Thrombelastography, Treatment Outcome, Factor IX pharmacology, Hemophilia B drug therapy, Recombinant Proteins pharmacology

Abstract

Baxter has developed a new recombinant factor IX (rFIX) drug product (BAX326) for treating patients with hemophilia B, or congenital FIX deficiency. An extensive preclinical program evaluated the pharmacokinetics, efficacy, and safety of BAX326 in different species. The efficacy of BAX326 was tested in three mouse models of primary pharmacodynamics: tail-tip bleeding, carotid occlusion, and thrombelastography. The pharmacokinetics was evaluated after a single intravenous bolus injection in mice, rats, and macaques. Toxicity was assessed in rats and macaques, safety pharmacology in rabbits and macaques, and immunogenicity in mice. BAX326 was shown to be efficacious in all three primary pharmacodynamic studies (P ≤ 0.0076). Hemostatic efficacy was dose related and similar for the three lots tested. Pharmacokinetic results showed that rFIX activity and rFIX antigen concentrations declined in a bi-phasic manner, similar to a previously licensed rFIX product. BAX326 was well tolerated in rabbits and macaques at all dose levels; no thrombogenic events and no adverse clinical, respiratory, or cardiovascular effects occurred. BAX326 was also shown to have a similar immunogenicity profile to the comparator rFIX product in mice. These results demonstrate that BAX326 has a favorable preclinical safety and efficacy profile, predictive of a comparable effect to that of the previously licensed rFIX in humans.

Published

2013

11. Towards a European strategy for medicines research (2014-2020): The EUFEPS position paper on Horizon 2020.

Author

Gaspar R, Aksu B, Cuine A, Danhof M, Takac MJ, Linden HH, Link A, Muchitsch EM, Wilson CG, Ohrngren P, and Dencker L

Subjects

Drug Industry, Europe, Public-Private Sector Partnerships, Universities, Biomedical Research, Drug Discovery

Abstract

As to the alignment of "Horizon 2020", ir is a more integrated approach to European science policy than expressed in the proposals previously drafted, and specifically considers: (i) promoting excellence in Science, (ii) establishing a sound industrial leadership and (iii) expressing an ambition to address current and future societal challenges. In this respect, the quest for a knowledge-based economy in Europe should result in proposals for industrial and employment policies that will consolidate the major European advantages in the biomedical, healthcare and pharmaceutical sectors. Horizon 2020 also provides the possibility of adopting a more flexible and simplified management route to drive European research through innovation, research and development. What should be additionally considered? Unmet medical needs, under pressure from demographic changes, await the generation of new medicines and health technologies which will evolve into a driver for a unified European policy. We believe that this should be focused on harnessing pharmaceutical knowledge for clinical use, as part of a response to accommodate patient needs and economic growth based on a robust, scientific approach. The bolder ambition for European research is to unlock key bottlenecks currently undermining European competitiveness. The historical lack of an appropriate business/innovation environment with reduced access to adequate risk finance instruments has severed the path for economic growth and industrial development. These issues are of critical importance and a solution is urgently needed to foster translation from the university to the healthcare sector through the generation and support of start-ups, spin-offs, university-industry consortia, and other platforms, which support translational research. The ultimate goal is implementation of holistic programmes: the 'bench to bedside' paradigm of medicines and other healthcare products. The European Research Council supports the basic biomedical research programmes of long term importance for development of medicines; however, fundamental research initiatives on medicines development will not be competitive in such an environment. In order to strengthen the long term outlook, we must foster innovative research within the university sector, EUFEPS proposes that a fund for such research be set up within Horizon 2020, which would be open for individual research groups and which would include Public-Public Partnerships (complementing already existing Public-Private Partnerships). How do we look for implementation? There is an established research agenda for medicines research that is globally focused, and which incorporates a cooperative model between universities and industry, facilitating integration of complex technologies. Regulatory Science will play an important role in this integration. This agenda uses tools arising from systems approaches (including discovery with systems biology and also systems pharmacology) and has the potential for providing better knowledge management, as well as technological innovation (including manufacturing). It also addresses the drive towards personalised medicines and can, with support from both public and private sectors, foster translation of knowledge to new technologies and from that, to new medicinal products and complex integrated systems. This is a part of a strategy capable of solving unmet medical needs, which would increase the quality of life of patients suffering from chronic and debilitating diseases. The instruments to allow the development of a research agenda should strengthen existing partnerships such as the IMI-JU model; allow for the creation of European-network infrastructures that can bring together existing competences with adequate European coordination, thus promoting advanced training and continuous professional development for the pharmaceutical sciences. This will be the cornerstone of a knowledge management strategy, providing education and training for healthcare professionals and scientists. A key role for EUFEPS is to help the research community to embrace these new holistic policies applied to the spectrum of pharmaceutical, medical and cognate sciences., (Copyright © 2012 Elsevier B.V. All rights reserved.)

Published

2012

12. A new mouse model mimicking thrombotic thrombocytopenic purpura: correction of symptoms by recombinant human ADAMTS13.

Author

Schiviz A, Wuersch K, Piskernik C, Dietrich B, Hoellriegl W, Rottensteiner H, Scheiflinger F, Schwarz HP, and Muchitsch EM

Subjects

ADAM Proteins administration & dosage, ADAMTS13 Protein, Animals, Body Weight drug effects, Dose-Response Relationship, Drug, Female, Hematocrit, Humans, Male, Mice, Mice, Inbred C57BL, Platelet Count, Purpura, Thrombotic Thrombocytopenic blood, Purpura, Thrombotic Thrombocytopenic pathology, Recombinant Proteins administration & dosage, Recombinant Proteins therapeutic use, Treatment Outcome, ADAM Proteins therapeutic use, Disease Models, Animal, Metalloendopeptidases genetics, Mice, Knockout, Purpura, Thrombotic Thrombocytopenic drug therapy, Purpura, Thrombotic Thrombocytopenic genetics

Abstract

Deficiency of a disintegrin and metalloproteinase with a thrombospondin type 1 motif, member 13 (ADAMTS13), a VWF-cleaving protease, is the key factor in the pathogenesis of thrombotic thrombocytopenic purpura (TTP), a life-threatening thrombotic microangiopathy. It is well established that ADAMTS13 deficiency results in elevated plasma levels of ultra-large VWF multimers (ULVWF), which are prone to induce platelet aggregation; however, the actual trigger of TTP development remains uncertain. Here we describe a new animal model in which some TTP-like symptoms can be triggered in ADAMTS13 knockout mice by challenge with 2000 units/kg body weight of recombinant human VWF containing ULVWF multimers. Animals rapidly showed clinical symptoms and developed severe thrombocytopenia. Schistocytosis, a decrease in hematocrit, and elevated serum lactate dehydrogenase levels were observed. The heart was identified as the most sensitive target organ with rapid onset of extensive platelet aggregation in the ventricles and myocardial necrosis. Prophylactic administration of 200 units/kg recombinant human ADAMTS13 protected ADAMTS13 knockout mice from developing TTP. Therapeutic administration of 320 units/kg rhADAMTS13 reduced the incidence and severity of TTP findings in a treatment interval-dependent manner. We therefore consider this newly established mouse model of thrombotic microangiopathy highly predictive for investigating the efficacy of new treatments for TTP.

Published

2012

13. BAX 855, a PEGylated rFVIII product with prolonged half-life. Development, functional and structural characterisation.

Author

Turecek PL, Bossard MJ, Graninger M, Gritsch H, Höllriegl W, Kaliwoda M, Matthiessen P, Mitterer A, Muchitsch EM, Purtscher M, Rottensteiner H, Schiviz A, Schrenk G, Siekmann J, Varadi K, Riley T, Ehrlich HJ, Schwarz HP, and Scheiflinger F

Subjects

Dose-Response Relationship, Drug, Drug Stability, Factor VIII pharmacokinetics, Half-Life, Hemophilia A metabolism, Humans, Recombinant Proteins administration & dosage, Recombinant Proteins chemistry, Recombinant Proteins pharmacokinetics, Drug Design, Factor VIII administration & dosage, Factor VIII chemistry, Hemophilia A drug therapy, Liposomes chemistry, Polyethylene Glycols chemistry

Abstract

A longer acting recombinant FVIII is expected to serve patients' demand for a more convenient prophylactic therapy. We have developed BAX 855, a PEGylated form of Baxter's rFVIII product ADVATE™ based on the ADVATE™ manufacturing process. The conjugation process for preparing BAX 855 uses a novel PEG reagent. The production process was adjusted to yield a rFVIII conjugate with a low PEGylation degree of about 2 moles PEG per FVIII molecule. This optimised modification degree resulted in an improved PK profile for rFVIII without compromising its specific activity. PEGylation sites were identified by employing various HPLC- and MS-based methods. These studies not only indicated that about 60% of the PEG chains are localised to the B-domain, which is cleaved off upon physiological activation during the coagulation process, but also demonstrated an excellent lot to lot consistency with regard to PEGylation site distribution. Detailed biochemical characterization further showed that PEGylated FVIII retained all the physiological functions of the FVIII molecule with the exception of binding to the LRP clearance receptor which was reduced for BAX 855 compared to ADVATE™. This might provide an explanation for the prolonged circulation time of BAX 855 as reduced receptor binding might slow-down clearance. Preclinical studies showed improved pharmacokinetic behaviour and clinically relevant prolonged efficacy compared to ADVATE™ without any signs of toxicity or elevated immunogenicity. The comprehensive preclinical data package formed the basis for approval of the phase 1 clinical study by European authorities which started in 2011.

Published

2012

14. Expression of recombinant human coagulation factors VII (rFVII) and IX (rFIX) in various cell types, glycosylation analysis, and pharmacokinetic comparison.

Author

Böhm E, Dockal M, Graninger M, Hasslacher M, Kaliwoda M, Konetschny C, Mitterer A, Muchitsch EM, Reiter M, and Scheiflinger F

Published

2011

15. Maintenance and break of immune tolerance against human factor VIII in a new transgenic hemophilic mouse model.

Author

van Helden PM, Unterthurner S, Hermann C, Schuster M, Ahmad RU, Schiviz AN, Weiller M, Antoine G, Turecek PL, Muchitsch EM, Schwarz HP, and Reipert BM

Subjects

Animals, Antibody Formation genetics, Antibody Formation physiology, Disease Models, Animal, Factor VIII antagonists & inhibitors, Female, Hemophilia A immunology, Hemophilia A pathology, Humans, Immune Tolerance physiology, Immunologic Memory physiology, Male, Mice, Mice, Inbred C57BL, Mice, Transgenic, Models, Biological, Species Specificity, Factor VIII genetics, Factor VIII immunology, Hemophilia A genetics, Immune Tolerance genetics, Immunologic Memory genetics

Abstract

Replacement of the missing factor VIII (FVIII) is the current standard of care for patients with hemophilia A. However, the short half-life of FVIII makes frequent treatment necessary. Current efforts focus on the development of longer-acting FVIII concentrates by introducing chemical and genetic modifications to the protein. Any modification of the FVIII protein, however, risks increasing its immunogenic potential to induce neutralizing antibodies (FVIII inhibitors), and this is one of the major complications in current therapy. It would be highly desirable to identify candidates with a high risk for increased immunogenicity before entering clinical development to minimize the risk of exposing patients to such altered FVIII proteins. In the present study, we describe a transgenic mouse line that expresses a human F8 cDNA. This mouse is immunologically tolerant to therapeutic doses of native human FVIII but is able to mount an antibody response when challenged with a modified FVIII protein that possesses altered immunogenic properties. In this situation, immunologic tolerance breaks down and antibodies develop that recognize both the modified and the native human FVIII. The applicability of this new model for preclinical immunogenicity assessment of new FVIII molecules and its potential use for basic research are discussed.

Published

2011

16. Biochemical, molecular and preclinical characterization of a double-virus-reduced human butyrylcholinesterase preparation designed for clinical use.

Author

Weber A, Butterweck H, Mais-Paul U, Teschner W, Lei L, Muchitsch EM, Kolarich D, Altmann F, Ehrlich HJ, and Schwarz HP

Subjects

Butyrylcholinesterase pharmacokinetics, Butyrylcholinesterase toxicity, Humans, Materials Testing, Organophosphates, Pharmacokinetics, Quality Control, Viruses, Butyrylcholinesterase isolation & purification, Drug Industry methods

Abstract

Background and Objectives: A human plasma-derived butyrylcholinesterase preparation manufactured on the industrial scale is described., Material and Methods: The human butyrylcholinesterase (hBChE) product was extensively investigated for its purity using immunological and electrophoretic methods and characterized by thorough glycoproteomic approaches. A comprehensive preclinical testing programme addressing safety and pharmacokinetic parameters supplemented the biochemical characterization., Results: The high-purity hBChE preparation is tetrameric and has high specific activity and molecular integrity of the protein backbone. Acute toxicity studies and in vivo thrombogenicity studies provided evidence of a sufficient safety margin for use in humans., Conclusion: Extensive preclinical safety and pharmacokinetic testing confirmed that this hBChE preparation can be used for further efficacy testing as a bioscavenger for toxic organophosphate compounds in appropriate animal models and ultimately in humans., (© 2010 Baxter Innovations GmBH. Vox Sanguinis © 2010 International Society of Blood Transfusion.)

Published

2011

17. Towards a standardization of the murine tail bleeding model.

Author

Greene TK, Schiviz A, Hoellriegl W, Poncz M, and Muchitsch EM

Subjects

Animals, Female, Hemostasis, Male, Mice, Species Specificity, Disease Models, Animal, Hemorrhage physiopathology, Tail blood supply

Published

2010

18. Preclinical testing of human recombinant von Willebrand factor: ADAMTS13 cleavage capacity in animals as criterion for species suitability.

Author

Muchitsch EM, Dietrich B, Rottensteiner H, Auer W, Nehrbass D, Gritsch H, Ehrlich HJ, Turecek PL, and Schwarz HP

Subjects

Animals, Humans, Recombinant Proteins pharmacology, ADAM Proteins metabolism, von Willebrand Factor pharmacology

Abstract

Von Willebrand factor (VWF) is cleaved by the plasma metalloprotease ADAMTS13 ( A Disintegrin and Metalloproteinase with Thrombo Spondin repeats, number 13) that regulates the hemostatic activity of VWF by limiting its multimeric size in the human system. In vitro and ex vivo studies have shown that human recombinant VWF (rVWF) is virtually resistant to the proteolytic activity of murine ADAMTS13. In contrast, rabbit and cynomolgus ADAMTS13 is able to cleave human rVWF. These findings were consistent with in vivo results showing distinct pharmacological behavior of human rVWF depending on the cleaving capacity of ADAMTS13 present in the species tested. Studies were performed using three mouse strains (ADAMTS13 deficient, C57BL/6J [wild type], VWF deficient), rats, rabbits, and cynomolgus monkeys. All animals were infused once with different doses of human rVWF and, in addition, 14 daily doses were given to rats and cynomolgus monkeys. Exaggerated pharmacological effects were observed in mice, with the ADAMTS13 knockout mouse being the most sensitive strain. Similar findings with decreased incidence and severity were seen in normal C57BL/6J mice and also in VWF-deficient mice, where they were least pronounced. In rats, exaggerated pharmacological effects were observed only after 14 doses. Rabbits and cynomolgus monkeys showed no exaggerated pharmacological effects. These differences between species and between mouse strains suggest that the efficiency of ADAMTS13 to cleave rVWF determines the severity of clinical, laboratory and pathohistological findings. These observations highlight the importance of evaluating species' suitability for the generation of meaningful preclinical data for determining the therapeutic safety margins for human patients. Only animals with a sufficient rVWF cleavage capacity by endogenous ADAMTS13 (rabbits and cynomolgus monkeys) are considered appropriate animal models for preclinical evaluation of the rVWF product.

Published

2010

19. Optimization, refinement and reduction of murine in vivo experiments to assess therapeutic approaches for haemophilia A.

Author

Baumgartner B, Jaki T, Wolfsegger MJ, Eder B, Schiviz A, Schwarz HP, and Muchitsch EM

Subjects

Animals, Arterial Occlusive Diseases chemically induced, Arterial Occlusive Diseases drug therapy, Arterial Occlusive Diseases pathology, Carotid Artery Diseases chemically induced, Carotid Artery Diseases drug therapy, Carotid Artery Diseases pathology, Chlorides toxicity, Disease Models, Animal, Female, Ferric Compounds toxicity, Hemophilia A chemically induced, Male, Mice, Mice, Inbred Strains, Mice, Knockout, Regional Blood Flow drug effects, Animal Use Alternatives, Animal Welfare, Coagulants pharmacology, Hemophilia A drug therapy, Research Design

Abstract

The tail cut bleeding model (CUT) is routinely used in factor VIII-deficient mice to assess pharmacodynamic effects of therapeutic strategies for haemophilia A. Results from this model are highly variable, many modifications to the model are reported and at times the animals' wellbeing may be compromised by recording survival as an endpoint. We therefore investigated if the ferric chloride carotid occlusion model (COM) used for thrombosis research can be applied to enhance data quality and animal welfare in haemophilia A research. Relative dose effects and relative dose variations were calculated for the CUT and COM. The requisite sample sizes were estimated and the importance of survival rates to assess rebleeds during recovery was evaluated by correlating initial blood loss to mortality. Relative dose effects increased with higher doses in both models. The COM was more sensitive at lower doses than the CUT, had up to 82% less variation across doses and clearly showed superior accuracy. Only 5% of the sample size required for the CUT would be needed to establish non-inferiority between a specific therapeutic dose in haemophilia A mice and healthy wild-type animals. A strong statistically significant correlation was found between initial blood loss and mortality within 24 h. Our findings clearly suggest that the COM is a valid tool for assessing haemophilia A treatment in vivo. The highly reproducible data means that significantly fewer animals are required and a more humane endpoint can be used by directly assessing clot stability instead of survival rate.

Published

2010

20. Modulation of factor VIII-specific memory B cells.

Author

Reipert BM, Allacher P, Hausl C, Pordes AG, Ahmad RU, Lang I, Ilas J, Windyga J, Klukowska A, Muchitsch EM, and Schwarz HP

Subjects

Adolescent, Adult, Animals, Antibodies immunology, Antigens, CD immunology, B-Lymphocytes cytology, CD40 Ligand immunology, Cell Differentiation, Child, Factor VIII administration & dosage, Factor VIII antagonists & inhibitors, Hemophilia A therapy, Humans, Lymphocyte Activation immunology, Mice, Spleen cytology, Spleen immunology, Young Adult, B-Lymphocytes immunology, Factor VIII immunology, Hemophilia A immunology, Immunologic Memory immunology

Abstract

The development of inhibitory antibodies against factor VIII (FVIII) is the major complication in patients with haemophilia A who are treated with FVIII products. Memory B cells play an essential role in maintaining established antibody responses. Upon re-exposure to the same antigen, they are rapidly re-stimulated to proliferate and differentiate into antibody-secreting plasma cells (ASC) that secrete high-affinity antibodies. It is, therefore, reasonable to believe that memory B cells have to be eradicated or inactivated for immune tolerance induction therapy to be successful in patients with haemophilia A and FVIII inhibitors. The aim of our studies was the development of strategies to prevent FVIII-specific memory B cells from becoming re-stimulated. We established a 6-day in vitro culture system that enabled us to study the regulation of FVIII-specific murine memory-B-cell re-stimulation. We tested the impact of the blockade of co-stimulatory interactions, of different concentrations of FVIII and of ligands for toll-like receptors (TLR). The blockade of B7-CD28 and CD40-CD40 ligand interactions prevented FVIII-specific murine memory B cells from becoming re-stimulated by FVIII in vitro and in vivo. Furthermore, high concentrations of FVIII blocked re-stimulation of FVIII-specific murine memory B cells. Triggering of TLR7 amplified re-stimulation by low concentrations of FVIII and prevented blockade by high concentrations of FVIII. We conclude that we defined modulators that either amplify or inhibit the re-stimulation of FVIII-specific murine memory B cells. Currently, we are investigating whether the same modulators operate in patients with haemophilia A and FVIII inhibitors.

Published

2010

21. Serum-derived immunoglobulins alter amyloid beta transport across a blood-brain barrier in vitro model.

Author

Poetsch V, Bennani-Baiti B, Neuhaus W, Muchitsch EM, and Noe CR

Subjects

Algorithms, Amyloid beta-Peptides analysis, Animals, Biological Transport, Active, Blotting, Western, Cell Line, Electrophoresis, Polyacrylamide Gel, Fluorescent Antibody Technique, Glycation End Products, Advanced metabolism, Humans, Immune Sera chemistry, Permeability, Rats, Receptors, Fc drug effects, Amyloid beta-Peptides metabolism, Blood-Brain Barrier drug effects, Blood-Brain Barrier metabolism, Immunoglobulins blood, Immunoglobulins pharmacology

Abstract

Since passive immunization with serum-derived immunoglobulins (intravenous immunoglobulins) showed several positive effects in some patients with Alzheimer's disease (AD), intravenous immunoglobulins (IVIG) are discussed as a possible treatment option. IVIG, an antibody product derived from human plasma, contains natural antibodies against amyloid beta(Abeta) peptide. Until now it is not known, how IVIG interferes with pathogenesis in AD, but several proposed mechanisms are in discussion. Receptor types which are involved in transport processes at the BBB are LRP, RAGE and hFcRn. We were looking for an in vitro BBB model expressing these receptors and studied the alteration of transport of Abeta peptides across this model under the influence of immunoglobulins. Cell line ECV304 was found to be suitable for our experiments. We found evidence for involvement of an improved clearance of Abeta across the BBB as well as a decreased Abeta influx from blood to the brain probably following complex formation of immunoglobulins with free Abeta in the periphery. Furthermore, we were able to confirm the activity of IVIG preparations which acted the same way but showed slightly less efficacy in comparison to monoclonal anti-Abeta antibodies. Based on these results we suggest multiple mechanisms responsible for the efficacy of immunotherapy in Alzheimer's disease.

Published

2010

22. Development of a plasma- and albumin-free recombinant von Willebrand factor.

Author

Turecek PL, Mitterer A, Matthiessen HP, Gritsch H, Varadi K, Siekmann J, Schnecker K, Plaimauer B, Kaliwoda M, Purtscher M, Woehrer W, Mundt W, Muchitsch EM, Suiter T, Ewenstein B, Ehrlich HJ, and Schwarz HP

Subjects

Albumins chemistry, Animals, Area Under Curve, CHO Cells, Cricetinae, Cricetulus, Disease Models, Animal, Dogs, Factor VIII metabolism, Half-Life, Humans, Mice, Mice, Knockout, Plasma chemistry, Recombinant Proteins genetics, Recombinant Proteins isolation & purification, Recombinant Proteins metabolism, Recombinant Proteins pharmacokinetics, Swine, von Willebrand Diseases drug therapy, von Willebrand Factor genetics, von Willebrand Factor isolation & purification, von Willebrand Factor metabolism, von Willebrand Factor pharmacokinetics, Recombinant Proteins chemistry, von Willebrand Factor chemistry

Abstract

Baxter has developed a recombinant therapy for treating von Willebrand's disease. Recombinant VWF is co-expressed with the rFVIII in CHO cells used to produce the rFVIII product Advate. This rVWF is used as a drug component for a rVWF-rFVIII complex drug product. CHO cells produce partially processed and partially un-processed rVWF still containing the pro-peptide. In order to make a consistent preparation containing mature and processed rVWF only rVWF is exposed to recombinant furin to remove the pro-peptide. Recombinant VWF and furin are produced under serum- and protein-free conditions. It is highly purified by a series of chromatographic steps and formulated in a protein-free buffer and has a homogeneous multimer distribution. The specific activity is higher in rVWF than in commercial plasma-derived VWF-FVIII complex products. SDS agarose electrophoretic analysis shows the presence of ultra-high molecular weight multimers. The FVIII-binding capacity and affinity of rVWF to FVIII is comparable to VWF in plasma. Carbohydrate analysis shows an intact glycosylation pattern. Recombinant VWF binds to collagen and promotes platelet adhesion under shear stress. It stabilizes endogenous FVIII in VWF-deficient knock-out mice as seen by a secondary rise in murine FVIII.

Published

2009

23. Species-dependent variability of ADAMTS13-mediated proteolysis of human recombinant von Willebrand factor.

Author

Varadi K, Rottensteiner H, Vejda S, Weber A, Muchitsch EM, Turecek PL, Ehrlich HJ, Scheiflinger F, and Schwarz HP

Subjects

ADAM Proteins blood, ADAMTS13 Protein, Animals, Blotting, Western, Humans, Hydrolysis, Macaca fascicularis, Mice, Rabbits, Recombinant Proteins metabolism, Species Specificity, ADAM Proteins metabolism, von Willebrand Factor metabolism

Abstract

Background: von Willebrand factor (VWF) is composed of a series of multimers, the sizes of which are regulated by the plasma metalloprotease ADAMTS13., Objective: Proteolysis of human recombinant VWF (rVWF) by ADAMTS13 present in the plasma of different species typically used as preclinical animal models was investigated to evaluate the efficacy and safety of rVWF., Methods: Degradation of rVWF was studied in vitro under moderate denaturing conditions and was monitored by multimer analysis, residual collagen binding, and immunoblot analysis. In vivo cleavage was determined by administration of rVWF to cynomolgus monkeys, rabbits and VWF-deficient mice and subsequent analysis of plasma samples by immunoblot. Plasma ADAMTS13 levels were determined with a synthetic human VWF peptide (FRETS-VWF73)., Results: From the animals tested, only rabbit plasma was as efficient as human plasma in proteolysing rVWF in vitro. Mouse plasma virtually failed to cleave rVWF. Administration of human rVWF resulted in ADAMTS13-specific cleavage products in rabbits and, to a lesser extent, in cynomolgus monkeys at various doses of rVWF. Virtually no cleavage occurred in mice. ADAMTS13 activity levels in rabbit and monkey plasma were similar to those in human plasma and were not significantly altered upon infusion of rVWF up to very high doses, indicating that rVWF did not lead to an exhaustion of endogenous ADAMTS13 in both species., Conclusions: The differences in susceptibility to cleavage of rVWF by different species need to be considered when interpreting the physiology of human rVWF from results of tests in animal models.

Published

2009

24. A guide to murine coagulation factor structure, function, assays, and genetic alterations.

Author

Emeis JJ, Jirouskova M, Muchitsch EM, Shet AS, Smyth SS, and Johnson GJ

Subjects

Animals, Blood Coagulation, Fibrinogen genetics, Hemostasis genetics, Humans, Mice, Models, Biological, Models, Genetic, Partial Thromboplastin Time, Prothrombin Time, Thrombosis genetics, Disease Models, Animal

Abstract

Murine blood coagulation factors and function are quite similar to those of humans. Because of this similarity and the adaptability of mice to genetic manipulation, murine coagulation factors and inhibitors have been extensively studied. These studies have provided significant insights into human hemostasis. They have also provided useful experimental models for evaluation of the pathophysiology and treatment of thrombosis. This review contains recommendations for obtaining, processing and assaying mouse blood hemostatic components, and it summarizes the extensive literature on murine coagulation factor structure and function, assays and genetic alteration. It is intended to be a convenient reference source for investigators of hemostasis and thrombosis.

Published

2007

25. Induction of immune tolerance by oral IVIG.

Author

Maier E, Reipert BM, Novy-Weiland T, Auer W, Baumgartner B, Muchitsch EM, Fiedler C, Grillberger L, and Schwarz HP

Subjects

Administration, Oral, Adoptive Transfer, Animals, Factor VIII immunology, Female, Humans, Immunoglobulin Fab Fragments pharmacology, Immunoglobulin Fc Fragments pharmacology, Immunoglobulins, Intravenous administration & dosage, Mice, Mice, Inbred BALB C, Rheumatoid Factor blood, Immune Tolerance drug effects, Immunoglobulins, Intravenous pharmacology

Abstract

In the last years evidence has been provided for the importance of B cells in the pathogenesis of rheumatoid arthritis (RA). Several studies have supported the concept that humoral immunity, manifested by the production of autoantibodies, such as rheumatoid factors (RFs), plays a significant role in the course of the disease. Specific targeting of autoantibody-producing B cells, such as RF-producing B cells, should therefore be a promising new approach in the treatment of RA. We used a mouse model to induce human RF responses and asked the question whether oral treatment with the antigen (human IgG) recognized by RFs could induce immune tolerance to RF responses. Balb/c mice were orally treated with polyvalent human IgG before and after immunization with insoluble immune complexes (ICs) that triggered the induction of RFs. Serum titers of RFs were significantly reduced after both primary and booster immunization when human IgG was given as a single oral dose or continuously in drinking water. Continuous treatment with human IgG even prevented booster effects on RFs when treatment started after primary immunization. Treatment with IgG fragments provided evidence that the observed effect of human IgG was mediated by the Fc part and not the Fab part of IgG. Furthermore, transfer of spleen cells obtained from mice after oral treatment with human IgG suppressed RF responses in recipient mice. These data give promising indications that oral human IgG might represent an alternative approach for immunosuppressive B-cell targeted therapies in RA.

Published

2007

26. A new liquid, intravenous immunoglobulin product (IGIV 10%) highly purified by a state-of-the-art process.

Author

Teschner W, Butterweck HA, Auer W, Muchitsch EM, Weber A, Liu SL, Wah PS, and Schwarz HP

Subjects

Animals, Dogs, Drug Evaluation, Preclinical, Drug-Related Side Effects and Adverse Reactions, Humans, Immunoglobulins, Intravenous chemistry, Immunoglobulins, Intravenous pharmacokinetics, Immunologic Factors chemistry, Immunologic Factors pharmacokinetics, Mice, Pharmaceutical Preparations blood, Pharmaceutical Preparations chemistry, Rabbits, Rats, Treatment Outcome, Decontamination methods, Disinfection methods, Immunoglobulins, Intravenous isolation & purification, Immunologic Factors isolation & purification, Pharmaceutical Preparations isolation & purification

Abstract

Background and Objectives: The ultimate goal was to generate an industrial-scale process suitable to produce a high-yield, safe and stable immunoglobulin G (IgG) preparation for intravenous administration, which is ready to use for customer convenience. This new liquid 10% IgG preparation (IGIV 10%) was compared to Gammagard SD, a licenced lyophilized immunoglobulin in biochemical and preclinical testing., Materials and Methods: The new process, which includes three dedicated virus clearance steps, is a streamlined combination of the currently applied and well-established manufacturing procedures. The biochemical characterization is done by standard methods focusing on purity, integrity and functionality of the preparation. Efficacy is demonstrated in vivo by mouse protection testing and in vitro by opsonization and protein A affinity chromatography. Pharmacokinetics in rats is evaluated after a single intravenous dose. The anaphylactoid potential is determined in rats and in guinea pigs, while thrombogenicity is assessed in a rabbit model. The influence of the products on vital functions is tested on dogs, while acute toxicity studies are carried out on mice and rats., Results: The biochemical characterization data demonstrate the high purity of monomeric IgG in the product. The mouse protection test showed that the protective activity against systemic bacterial infections of IGIV 10% is at least as good as the reference Gammagard SD. This result is supported by the broad spectrum of antibodies in high titres against bacteria and viruses and the high functional integrity of the IgG molecule (> or = 90% functionally intact IgG) in IGIV 10%. The opsonic activity of all IGIV 10% lots is similar to the one of the reference Gammagard SD. In safety and thrombogenicity studies, no adverse effects of IGIV 10% were observed. Pharmacokinetic studies showed no statistically significant differences between the two products. In the acute toxicity animal studies, IGIV 10% compared favourably to the reference Gammagard SD., Conclusions: The new manufacturing process enables the production of a highly purified IgG preparation for intravenous administration. The product has an IgG subclass distribution similar to plasma and contains a broad spectrum of functionally intact antibodies. Preclinical studies demonstrate that the liquid IGIV 10% combines excellent qualities of efficacy, safety and tolerability.

Published

2007

27. Liver expression of hepcidin and other iron genes in two mouse models of beta-thalassemia.

Author

De Franceschi L, Daraio F, Filippini A, Carturan S, Muchitsch EM, Roetto A, and Camaschella C

Subjects

Animals, Disease Models, Animal, Female, Gene Expression Regulation, Hepcidins, Iron metabolism, Iron Overload genetics, Iron Overload metabolism, Mice, Mice, Inbred C57BL, Mice, Inbred DBA, Mice, Knockout, Mice, Mutant Strains, Antimicrobial Cationic Peptides biosynthesis, Antimicrobial Cationic Peptides genetics, Liver metabolism, beta-Thalassemia genetics, beta-Thalassemia metabolism

Abstract

Background and Objectives: Homozygous beta-thalassemia patients may develop iron overload even if untransfused, due to inappropriately high intestinal iron absorption. Reduction of hepcidin synthesis has been reported both in patients and in animal models. We have measured liver hepcidin and other iron gene transcripts in two different mouse models of beta-thalassemia at different ages., Design and Methods: Mice Hbb(th/th), characterized by spontaneous homozygous deletion of the major b1 globin gene were studied at 2 and 8 months. Mice Hbb(th/3+), characterized by the heterozygous deletion of b1 and b2 globin genes were studied at 4 and 10 months. Hematologic data were obtained and iron overload estimated by Perls' staining of the liver. Expression of liver hepcidin, Tfr2, Hjv, Fpn and Hfe RNA was assessed by real-time polymerase chain reaction. Levels of serum cytokines (interleukin-6, IL-1beta, IL-10, granulocyte-macrophage colony-stimulating factor) levels were assayed by enzyme-linked immunosorbent assay., Results: Hemoglobin, hematocrit and mean corpuscular volume were significantly reduced in both beta-thalassemia models, more significantly in Hbb(th/3+), which have the greater, age-dependent, iron overload. Hepcidin RNA was not increased despite iron overload in both strains. Fpn RNA was increased and Tfr2 was decreased in older animals. Inflammatory cytokine levels were striking variable and unrelated to hepcidin levels., Interpretation and Conclusions: Although anemia is reported to inhibit hepcidin expression, normal hepcidin synthesis was maintained in both thalassemic models studied. However, hepcidin levels were inappropriate for the body iron, especially in Hbb(th/3+) 10-month-old animals. As we previously reported in wild type mice after parenteral iron overload, Tfr2 is reduced and Fpn RNA increased in thalassemic mice. Inflammatory cytokines did not play a major role in increasing hepcidin levels or in modifying iron homeostasis in this study.

Published

2006

28. Protective effects of S-nitrosoalbumin on lung injury induced by hypoxia-reoxygenation in mouse model of sickle cell disease.

Author

de Franceschi L, Malpeli G, Scarpa A, Janin A, Muchitsch EM, Roncada P, Leboeuf C, Corrocher R, Beuzard Y, and Brugnara C

Subjects

Animals, Animals, Genetically Modified, Disease Models, Animal, Drug Evaluation, Female, Hemodynamics drug effects, Male, Matrix Metalloproteinase 9 metabolism, Mice, Mice, Inbred C57BL, Nitroso Compounds therapeutic use, Platelet Aggregation drug effects, Serum Albumin, Bovine therapeutic use, Anemia, Sickle Cell complications, Hypoxia complications, Nitroso Compounds pharmacology, Pulmonary Veno-Occlusive Disease prevention & control, Reperfusion Injury complications, Serum Albumin, Bovine pharmacology

Abstract

Nitric oxide (NO) is a potential new therapeutic agent for sickle cell disease (SCD). We investigated the effects of NO donor on hypoxia-induced acute lung injury that occurs when transgenic sickle cell SAD mice are exposed to chronic hypoxia, a model for lung vasoocclusive sickle cell events. In wild-type and SAD mice, intraperitoneal injection of S-nitrosoalbumin (NO-Alb) produced no significant hematologic changes under room air conditions, whereas it induced mild temporary hypotension and inhibition of platelet aggregation. NO-Alb administration (300 mg/kg ip twice a day, equivalent to 7.5 microM NO) in wild-type and SAD mice exposed to 46 h of hypoxia (8% oxygen) followed by 2 h of normoxia resulted in 1) reduction of the hypoxia-induced increase in blood neutrophil count, 2) prevention of hypoxia-induced increased IL-6 and IL-1beta levels in bronchoalveolar lavage, 3) reduction of the lung injury induced by hypoxia-reoxygenation, 4) prevention of thrombus formation, and 5) prevention of hypoxia-induced increase of lung matrix metalloproteinase-9 gene expression. These effects provide new insights into the possible use of NO-Alb in the treatment of acute lung injury in SCD.

Published

2006

29. Preventing restimulation of memory B cells in hemophilia A: a potential new strategy for the treatment of antibody-dependent immune disorders.

Author

Hausl C, Ahmad RU, Schwarz HP, Muchitsch EM, Turecek PL, Dorner F, and Reipert BM

Subjects

Animals, Antibodies metabolism, Antibody Specificity, Antigens, CD immunology, Antigens, CD metabolism, B-Lymphocytes cytology, B-Lymphocytes metabolism, B7-1 Antigen immunology, B7-1 Antigen metabolism, B7-2 Antigen, Bone Marrow Cells cytology, Bone Marrow Cells immunology, Bone Marrow Cells metabolism, CD40 Antigens immunology, CD40 Antigens metabolism, CD40 Ligand immunology, CD40 Ligand metabolism, Cell Differentiation immunology, Cytokines metabolism, Factor VIII genetics, Factor VIII immunology, Hemophilia A genetics, Humans, Immunoglobulin G blood, Immunoglobulin G immunology, Lymphocyte Activation immunology, Male, Membrane Glycoproteins immunology, Membrane Glycoproteins metabolism, Mice, Mice, Inbred C57BL, Receptors, Antigen, B-Cell immunology, Receptors, Antigen, B-Cell metabolism, Recombinant Proteins genetics, Recombinant Proteins immunology, Spleen cytology, T-Lymphocytes immunology, T-Lymphocytes metabolism, Antibodies immunology, B-Lymphocytes immunology, Hemophilia A immunology, Immunologic Memory immunology

Abstract

Memory B cells are responsible for the rapidly emerging antibody response after antigen reexposure. The signals required for the restimulation of memory B cells have not been fully explained. We used a murine model of anti-factor VIII (FVIII) antibody responses in hemophilia A to study the requirements for the restimulation of FVIII-specific memory B cells and their differentiation into anti-FVIII antibody-producing cells. We were particularly interested in the significance of activated T cells and costimulatory interactions. Our results indicate that the restimulation of FVIII-specific memory B cells is strictly dependent on interactions with activated T cells. These activated T cells can be specific for either FVIII or third-party antigens. Restimulation by T cells specific for third-party antigens requires the presence of FVIII, indicating that signals induced by B-cell receptor (BCR) triggering and by interactions with activated T cells are important. The blockade of B7-1 or B7-2 as well as the blockade of CD40L inhibits the restimulation and differentiation of FVIII-specific memory B cells in vitro and in vivo. The interference with inducible costimulator-inducible costimulator ligand (ICOS-ICOSL) interactions, however, does not cause any modulation. As expected, the production of anti-FVIII antibodies by plasma cells is not dependent on any of the costimulatory interactions tested.

Published

2004

30. Effects of alpha1-acid glycoprotein in combination with catecholamines on hemorrhagic hypovolemic shock in rats.

Author

Muchitsch EM, Pichler L, and Schwarz HP

Subjects

Animals, Blood Pressure drug effects, Cardiac Output drug effects, Cardiotonic Agents therapeutic use, Dopamine therapeutic use, Dose-Response Relationship, Drug, Drug Combinations, Fluid Therapy, Heart Rate drug effects, Humans, Male, Norepinephrine therapeutic use, Rats, Rats, Sprague-Dawley, Resuscitation, Shock, Hemorrhagic physiopathology, Stroke Volume drug effects, Vascular Resistance drug effects, Vasoconstrictor Agents therapeutic use, Catecholamines pharmacology, Orosomucoid pharmacology, Shock, Hemorrhagic drug therapy

Abstract

To determine whether the beneficial effects of catecholamines on the variables of hemorrhagic hypovolemic shock are augmented by coadministration of alpha1-acid glycoprotein during resuscitation, alpha1-acid glycoprotein (200 mg/kg), a placebo formulation or Ringer's solution was infused in a rat model of hemorrhagic hypovolemic shock for 1 h concomitantly with either norepinephrine (CAS 51-40-1; 0.1, 0.3, 1 microg x kg(-1) x min(-1)) or dopamine (CAS 62-31-7; 5, 10, 15 microg x kg(-1) x min(-1)). Resuscitation with norepinephrine or dopamine alone was continued for a further 4 h. Mean arterial blood pressure, cardiac output, stroke volume, heart rate and total peripheral vascular resistance were measured during the entire 5-h period. The combination of dopamine or norepinephrine with alpha1-acid glycoprotein more effectively restored mean arterial blood pressure and cardiac output than analogous combinations with placebo formulation or Ringer's solution. So co-administration with alpha1-acid glycoprotein considerably augments the beneficial effects of catecholamines on the main variables of hemorrhagic hypovolemic shock.

Published

2004

31. Beneficial effect of albumin therapy attributable to alpha1-acid glycoprotein?

Author

Muchitsch EM and Schwarz HP

Subjects

Animals, Brain Ischemia drug therapy, Humans, Infarction, Middle Cerebral Artery drug therapy, Rats, Albumins therapeutic use, Orosomucoid physiology, Stroke drug therapy

Published

2003

32. Recombinant von Willebrand factor-insight into structure and function through infusion studies in animals with severe von Willebrand disease.

Author

Schwarz HP, Schlokat U, Mitterer A, Váradi K, Gritsch H, Muchitsch EM, Auer W, Pichler L, Dorner F, and Turecek PL

Subjects

Animals, Dimerization, Disease Models, Animal, Dogs, Factor VIII drug effects, Factor VIII metabolism, Humans, Infusions, Parenteral, LDL-Receptor Related Protein-Associated Protein, Low Density Lipoprotein Receptor-Related Protein-1, Mice, Mice, Knockout, Protein Precursors administration & dosage, Protein Precursors metabolism, Protein Precursors pharmacokinetics, Recombinant Proteins administration & dosage, Recombinant Proteins pharmacology, Structure-Activity Relationship, von Willebrand Diseases metabolism, von Willebrand Factor administration & dosage, Molecular Probe Techniques, von Willebrand Diseases drug therapy, von Willebrand Factor pharmacology

Abstract

We used a canine and a murine model of von Willebrand disease (vWD) to study the in vivo effects of recombinant von Willebrand factor (vWF). Two preparations were used: (1) a fully processed mature vWF; this was achieved by coexpression of furin. (2) A preparation containing unprocessed pro-vWF, the propeptide still covalently linked to mature vWF. Both preparations induced an increase in canine and murine factor VIII:C (FVIII), which was sustained even when vWF antigen had been removed from the circulation. vWF multimers were analyzed in the plasma samples after infusion using ultra high-resolution 3% agarose gels to allow the separation of homoforms and heteroforms of the vWF polymers. Administration of pro-vWF to dogs with severe vWD resulted in the removal of the propeptide and maturation of vWF in the circulation, indicating that the propeptide cleavage from unprocessed vWF can occur extracellularly. This suggests that the vWF propeptide, besides being derived from the Weibel-Palade bodies of endothelial cells after stimulation, can also be cleaved by pro-vWF in plasma. Using a murine model of vWD, the involvement of the low-density lipoprotein receptor-related protein (LRP) in the clearance of FVIII was established. The low levels of FVIII observed in the absence of vWF are due to an enhanced clearance of FVIII by binding to LRP and removal from the circulation through endocytosis. Administration of the receptor-associated protein (RAP) as a recombinant fusion protein to vWF knockout mice significantly improved the in vivo recovery of recombinant FVIII and the survival time of otherwise rapidly cleared FVIII.

Published

2002

33. Effects of alpha 1-acid glycoprotein on acute pancreatitis and acute lung injury in rats.

Author

Muchitsch EM, Varadi K, and Pichler L

Subjects

Acute Disease, Animals, Bronchoalveolar Lavage Fluid cytology, Ceruletide, Edema chemically induced, Edema prevention & control, Glycodeoxycholic Acid, Hemorrhage chemically induced, Hemorrhage pathology, Lipopolysaccharides, Lung Diseases chemically induced, Male, Pancreatitis chemically induced, Rats, Rats, Sprague-Dawley, Respiratory Tract Diseases chemically induced, Respiratory Tract Diseases drug therapy, Lung Diseases drug therapy, Orosomucoid therapeutic use, Pancreatitis drug therapy

Abstract

alpha 1-Acid glycoprotein (AAG), a highly negatively charged glycoprotein, well known for its capillary stabilizing effect, was tested in rat models of acute edematous pancreatitis, acute hemorrhagic-necrotizing pancreatitis, and acute respiratory distress syndrome (ARDS). In cerulein-elicited edematous pancreatitis AAG improved histological alterations at 200 mg/kg i.v. and plasma amylase activity at 1800 or 4200 mg/kg i.v. All other parameters (edema, plasma lipase) were not affected in a biologically relevant manner. In glycodeoxycholic acid-induced hemorrhagic-necrotizing pancreatitis AAG was without effect on parameters measured (plasma amylase, plasma lipase activity, histological scores) at 1800 or 4200 mg/kg i.v. At the extremely high dose of 1500 mg/kg i.v. plasma amylase and lipase levels were decreased. In lipopolysaccharide-mediated ARDS, AAG was tested at 50, 200 or 600 mg/kg i.v. AAG, but also the placebo formulation decreased the myeloperoxidase content in the bronchoalveolar lavage fluid. Histological alterations were improved by AAG, however, not by the placebo formulation. Lung water content was not significantly influenced by AAG, whereas Evans blue extravasation was significantly diminished by all three doses of AAG. It is concluded that the edematous pancreatitis is the first in vivo condition with increased extravascular fluid accumulation, in which AAG is not effective. Based on data presented here and literature data, there is evidence for a beneficial effect of AAG in acute lung injury.

Published

2000

34. Phenotypic expression of murine hemophilia.

Author

Muchitsch EM, Turecek PL, Zimmermann K, Pichler L, Auer W, Richter G, Gritsch H, and Schwarz HP

Subjects

Animals, Mice, Mice, Inbred C57BL, Factor VIII genetics, Hemophilia A genetics, Hemophilia A physiopathology, Mice, Knockout

Published

1999

35. [Preclinical investigation of alpha 1-acid glycoprotein (orosomucoid)].

Author

Pichler L, Muchitsch EM, and Schwarz HP

Subjects

Animals, Anti-Inflammatory Agents pharmacology, Anti-Inflammatory Agents therapeutic use, Brain drug effects, Capillary Permeability drug effects, Cerebrovascular Disorders complications, Drug Evaluation, Preclinical, Edema etiology, Edema prevention & control, Guinea Pigs, Neutrophils drug effects, Orosomucoid therapeutic use, Rats, Orosomucoid pharmacology

Abstract

The molecular properties of alpha 1-acid glycoprotein are briefly discussed. This molecule has been shown in in vitro experiments to have both a stabilizing effect on vascular permeability and antiinflammatory properties. We were able to demonstrate these two effects in vivo in guinea pigs (skin, Evan's Blue extravasation) and in rats (paw, carrageenan induced inflammation). Further experiments were performed in rats relating to possible therapeutic indications for alpha 1-acid glycoprotein: (1) inhibitory effect on brain edema formation after experimental stroke, (2) therapeutic effect in the puromycin aminonucleoside-induced minimal change nephrosis, (3) improvement of vital parameters in hemorrhagic-hypovolemic shock, (4) increase in survival rate in septic peritonitis, and (5) promising effects in burn-induced remote lung injury. The high content of sialic acid and the high negative charge of alpha 1-acid glycoprotein are believed to be major contributors to its stabilizing effect on vascular permeability. The protein is bound to the glycocalyx of the endothelial cells (and presumably to structures of the glomerular basement membrane), thereby hindering the passage of other polyanionic molecules through the vascular wall. The antiinflammatory/immunomodulatory effect of alpha 1-acid glycoprotein appears mainly due to suppression of polymorphonuclear neutrophils. This action is dependent on the glycan part of the molecule, which is highly variable (microheterogeneity). It is obvious that there are differences between the different glycan forms as far as the antiinflammatory property of the protein is concerned. Together with data in the literature, the results presented here suggest a variety of potential indications for therapeutic use of alpha 1-acid glycoprotein in humans.

Published

1999

36. Studies on the effect of human lys-plasminogen in a rat model of global cerebral ischemia.

Author

Auer W, Muchitsch EM, Philapitsch A, Pichler L, and Schwarz HP

Subjects

Animals, Body Water metabolism, Brain Chemistry drug effects, Brain Edema pathology, Brain Ischemia pathology, Brain Ischemia physiopathology, Carotid Arteries physiology, Fibrin metabolism, Fibrinolytic Agents blood, Humans, Male, Rats, Rats, Sprague-Dawley, Reperfusion Injury pathology, Brain Ischemia drug therapy, Peptide Fragments therapeutic use, Plasminogen therapeutic use

Abstract

Human lys-plasminogen and the corresponding formulation buffer were tested in a rat model of global cerebral ischemia (clamping of both carotid arteries, withdrawal of 5 ml blood for 30 min). The two main parameters, tested in different experimental set-ups, were 1. brain edema (water content) 23.5 h after reperfusion and 2. assessment of neurological deficits 24, 48 and 72 h after reperfusion. In some groups of animals of the first set-up, brains were examined histologically for microvascular fibrin deposits. In a separate group of animals the fibrinolytic plasma activity of rats treated with 500 CU/kg lys-plasminogen was studied. Concerning brain water content lys-plasminogen completely antagonized the formation of brain edema when given with 500 caseolytic Units (CU)/kg i.v. with blood reperfusion and was still effective when given 30 min later. 200 CU/kg i.v. given with blood reperfusion as well as 500 CU/kg i.v. given 60 min after blood reperfusion proved ineffective. In none of the brains investigated microvascular fibrin deposits were found. In experiments with assessment of neurological deficits, animals treated with 500 CU/kg lys-plasminogen i.v. showed almost no disabilities (like sham operated animals) when compared to ischemic (positive) controls which were rather severely handicapped. The formulation buffer of lys-plasminogen, tested in an equivalent volume, was without any effect in both set-ups. No fibrinolytic activity was found in plasma samples of rats up to 240 min after treatment with 500 CU/kg lys-plasminogen i.v. It is concluded from these experiments that human lys-plasminogen has a protective effect in rats against the sequelae of global cerebral ischemia which is not related to the well-known fibrinolytic potential but might be a separate quality.

Published

1997

37. In vivo effect of alpha 1-acid glycoprotein on experimentally enhanced capillary permeability in guinea-pig skin.

Author

Muchitsch EM, Teschner W, Linnau Y, and Pichler L

Subjects

Animals, Dose-Response Relationship, Drug, Drug Antagonism, Evans Blue, Guinea Pigs, Histamine pharmacology, Male, Plasminogen pharmacology, Skin drug effects, Capillary Permeability drug effects, Orosomucoid pharmacology, Skin blood supply

Abstract

Anesthetized guinea-pigs were intravenously injected with Evans blue. After intracutaneous injection of agonists (lys-plasminogen, histamine, platelet-activating factor, thrombin, bradykinin), the resulting wheals appeared blue in a dose-dependent manner, due to an enhanced capillary permeability, alpha 1-Acid glycoprotein, given i.v. in different doses (3.125-50 mg/kg) and at different times (30-180 min) before Evans blue administration, antagonized the effects of all agonists listed above. This was shown by a parallel shift of the agonist dose-response curves to the right. The effect was time-dependent (tmax: mainly 120 min) and dose-dependent. alpha 1-Acid glycoprotein antagonized the agonists in the following order: lys-plasminogen > histamine = platelet-activating factor > thrombin > bradykinin. As all agonist mentioned are suggested to play a major role in the shock-related increase in vascular permeability, a putatively beneficial role of alpha1-acid glycoprotein in shock is discussed.

Published

1996