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9. Immunogenicity of mAbs in non-human primates during nonclinical safety assessment

Author

van Meer, P.J.K., Kooijman, M., Brinks, V., Gispen-de Wied, C.C., Silva-Lima, B., Moors, E.H.M., Schellekens, H., Innovation Studies, Pharmaceutics, Sub Drug targeting, Section Innovation Studies, Sub Biotechnological drugs, and Innovation and Sustainability

Subjects
Taverne
Abstract

The immunogenicity of biopharmaceuticals used in clinical practice remains an unsolved challenge in drug development. Non-human primates (NHPs) are often the only relevant animal model for the development of monoclonal antibodies (mAbs), but the immune response of NHPs to therapeutic mAbs is not considered to be predictive of the response in humans because of species differences. In this study, we accessed the drug registration files of all mAbs registered in the European Union to establish the relative immunogenicity of mAbs in NHPs and humans. The incidence of formation of antidrug-antibodies in NHPs and patients was comparable in only 59% of the cases. In addition, the type of antidrug-antibody response was different in NHP and humans in 59% of the cases. Humanization did not necessarily reduce immunogenicity in humans. Immunogenicity interfered with the safety assessment during non-clinical drug development when clearing or neutralizing antibodies were formed. While important to interpret the study results, immunogenicity reduced the quality of NHP data in safety assessment. These findings confirm that the ability to compare relative immunogenicity of mAbs in NHPs and humans is low. Furthermore, immunogenicity limits the value of informative NHP studies.

Published
2013

10. Quality of Original and Biosimilar Epoetin Products

Author

Brinks, V., Hawe, A., Basmeleh, A.H.H., Joachin-Rodriguez, L., Haselberg, R., Somsen, G.W., Jiskoot, W., Schellekens, H., Advanced drug delivery systems/drug targeting, Biomolecular Analysis, Innovation Studies, Farmaceutische Analyse, Pharmaceutics, Sub Biotechnological drugs, Sub Biomolecular analysis, Dep Farmaceutische wetenschappen, BioAnalytical Chemistry, AIMMS, Advanced drug delivery systems/drug targeting, Biomolecular Analysis, Innovation Studies, Farmaceutische Analyse, Pharmaceutics, Sub Biotechnological drugs, Sub Biomolecular analysis, and Dep Farmaceutische wetenschappen

Subjects
protein characterization, Drugmisbruik en verslaving, Therapeutic equivalency, media_common.quotation_subject, Pharmacology toxicology, Pharmaceutical Science, Enzyme-Linked Immunosorbent Assay, Pharmacology, immunogenicity, Biomedische technologie en medicijnen, Farmacie/Biofarmaceutische wetenschappen (FARM), Mice, Pharmaceutical technology, hemic and lymphatic diseases, Medical technology, Animals, Protein Isoforms, Medicine, Potency, Quality (business), Pharmacology (medical), Bescherming en bevordering van de menselijke gezondheid, recombinant human erythropoietin, Erythropoietin, media_common, Biological Products, business.industry, Organic Chemistry, Farmacie(FARM), Electrophoresis, Capillary, Biosimilar, Recombinant Proteins, Therapeutic Equivalency, Chromatography, Gel, Molecular Medicine, Electrophoresis, Polyacrylamide Gel, Public Health, biosimilar, business, Analytical chemistry, Research Paper, medicine.drug, Biotechnology
Abstract

Purpose To compare the quality of therapeutic erythropoietin (EPO) products, including two biosimilars, with respect to content, aggregation, isoform profile and potency. Methods Two original products, Eprex (epoetin alfa) and Dynepo (epoetin delta), and two biosimilar products, Binocrit (epoetin alfa) and Retacrit (epoetin zeta), were compared using (1) high performance size exclusion chromatography, (2) ELISA, (3) SDS-PAGE, (4) capillary zone electrophoresis and (5) in-vivo potency. Results Tested EPO products differed in content, isoform composition, and potency. Conclusion Of the tested products, the biosimilars have the same or even better quality as the originals. Especially, the potency of originals may significantly differ from the value on the label.

Published
2011
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11. Hybrid transgenic immune tolerant mouse model for assessing the breaking of B cell tolerance by human interferon beta

Author

van Beers, M.M.C., Sauerborn, M.S., Gili, F., Hermeling, S., Brinks, V., Schellekens, H., Jiskoot, W., Advanced drug delivery systems/drug targeting, Innovation Studies, Pharmaceutics, Dep Farmaceutische wetenschappen, Sub Biotechnological drugs, and Section Innovation Studies

Subjects
Pharmacology, Medical technology, Farmacie(FARM), Biomedische technologie en medicijnen
Abstract

To date, the therapeutic efficacy of recombinant human proteins is limited by their potential to break B cell tolerance in patients. The formation of neutralising antibodies (NABs) directed against recombinant human interferon beta (rhIFNβ) is associated with a decrease in the therapeutic effect of the protein. For this reason, there is a need to study factors that can cause the immunogenicity of rhIFNβ. Transgenic C57Bl/6 mice that are immune tolerant for human interferon beta (hIFNβ) have been employed in a mouse model for assessing the breaking of immune tolerance by rhIFNβ. In this study, we used the original C57Bl/6 mouse model as well as the hybrid offspring from crossings of transgenic C57Bl/6 mice with wildtype FVB/N mice to study the immunogenicity of three commercial rhIFNβ products, Rebif®, Avonex® and Betaferon®. As determined by ELISA, wildtype C57Bl/6 mice failed to form binding antibodies (BABs) against Rebif® and Avonex® formulated with human serum albumin. Because not all interferon beta products induce antibodies in wildtype C57Bl/6 mice, the transgenic C57Bl/6 mice cannot be used to study the breaking of tolerance by these products. However, the crossing of transgenic C57Bl/6 mice with FVB/N mice resulted in wildtype hybrid offspring in which all products were immunogenic and transgenic hybrid offspring that showed immune tolerance for hIFNβ. Thus, these C57Bl/6 × FVB/N hybrid transgenic mice can be used to study the breaking of immune tolerance for all rhIFNβ products. Of the three products, only Betaferon® was able to break immune tolerance in the transgenic hybrids. With an MxA gene expression inhibition assay, NABs were detected in Betaferon® treated wildtype hybrid mice, but not in transgenic hybrid mice, indicating a distinct immune mechanism in wildtype and transgenic mice. A pegylated rhIFNβ-1a variant, PEG-rhIFNβ-1a, induced antibodies in wildtype hybrid mice, but did not break the immune tolerance of transgenic hybrid mice. This suggests that pegylation did not affect the potential of rhIFNβ-1a to break B cell tolerance.

Published
2010

12. Immunological mechanism underlying the immune response to tecombinant human protein therapeutics

Author

Sauerborn, M.S., Brinks, V., Jiskoot, W., Schellekens, H., Advanced drug delivery systems/drug targeting, Innovation Studies, Pharmaceutics, Dep Farmaceutische wetenschappen, and Section Innovation Studies

Subjects
Pharmacology, Medical technology, Farmacie(FARM), Biomedische technologie en medicijnen
Abstract

Recombinant human (rhu) protein therapeutics are powerful tools to treat several severe diseases such as multiple sclerosis and diabetes mellitus, among others. A major drawback of these proteins is the production of anti-drug antibodies (ADAs). In some cases, these ADAs have neutralizing capacity and can interfere with the efficacy and safety of the drug. Little is known about the immunological mechanisms underlying the unwanted immune response against human homolog protein therapeutics. This article aims to provide current insights into recent immunological developments and to link this with regard to production of ADAs. A particular focus is given to aggregates being present in a rhu protein formulation and their impact on the immune system, subsequently leading to breakage of tolerance and formation of ADAs. Aggregation is one of the key factors in immunogenicity and by reducing aggregation one can reduce immunogenicity and make drugs safer and more efficient.

Published
2010

13. Stress, emotion and cognition : role of mineralo- and glucocorticoid receptors

Author

Brinks, V., Oitzl, M.S., Kloet, E.R. de, and Leiden University

Subjects
Emotion, Cognition, Stress, Mineralo and glucocorticoid receptors
Abstract

Een emotionele gebeurtenis zoals een auto-ongeluk of eerste kus wordt goed onthouden. Stresshormonen spelen een grote rol bij deze link tussen emotie en cognitie. Onder normale omstandigheden worden emotionele en cognitieve processen bevorderd door stresshormonen zoals adrenaline en corticostero_den. Echter, te veel of juist te weinig stresshormonen, of een te lange periode van stress kan emotie en cognitie zo be_nvloeden dat sommige mensen stressgerelateerde ziekten zoals posttraumatische stressstoornis (PTSS) ontwikkelen. Waarom de een wel en de ander niet ziek wordt van stress is niet bekend. Men denkt dat de corticostero_den hiervoor van belang zijn. Vera Brinks richtte zich in haar onderzoek op de rol van corticostero_den in de integratie van emotionele en cognitieve processen, en dus stressgerelateerde fysiologie en psychopathologie. De focus lag hierbij op de rol van de corticostero_d receptoren in de hersenen; de mineralo- (MR) en glucocortico_d receptoren (GR). Dit onderzoek verrichte zij bij muizen. De experimenten lieten zien dat emotie een flinke verbetering van cognitieve prestaties gaf bij de muizen. Hierbij bleek dat activering van de GR - in vergelijking met MR activatie - belangrijk is in de integratie van emotie en cognitie. GR activatie met hoeveelheden van het stress hormoon corticosteron die ook vrij komen bij milde stress, resulteert in een optimale prestatie wanneer het dier ook een emotionele ervaring had. Een te lage of te hoge activatie van deze receptor (de GR) verstoorde de integratie van emotie en cognitie. Die GR werkt dus optimaal binnen nauwe grenzen. Wanneer de MR genetisch wordt 'uitgeschakeld'(knockout), dan worden bepaalde negatieve ervaringen niet uitgedoofd (vergeten). Een belangrijke vinding was ook dat corticostero_dbehandeling de herinnering aan een traumatische gebeurtenis zowel kan verminderen als verbeteren afhankelijk van de genetische achtergrond van de muizen Deze kennis kan gebruikt worden bij de behandeling van het veel te sterke geheugen voor traumatische en angstige PTSS-pati_nten. Bovendien is het een basis om de genetische factoren te onderzoeken die bij kunnen dragen aan het ontstaan en de vermindering van het sterke angstgeheugen bij PTSS-pati_nten. Onze experimenten hebben laten zien dat de MR een uitstekende kandidaat is als target voor een geheel nieuw soort geneesmiddelen.

Published
2009

14. Immunogenicity of mAbs in non-human primates during nonclinical safety assessment

Author

Innovation Studies, Pharmaceutics, Sub Drug targeting, Section Innovation Studies, Sub Biotechnological drugs, Innovation and Sustainability, van Meer, P.J.K., Kooijman, M., Brinks, V., Gispen-de Wied, C.C., Silva-Lima, B., Moors, E.H.M., Schellekens, H., Innovation Studies, Pharmaceutics, Sub Drug targeting, Section Innovation Studies, Sub Biotechnological drugs, Innovation and Sustainability, van Meer, P.J.K., Kooijman, M., Brinks, V., Gispen-de Wied, C.C., Silva-Lima, B., Moors, E.H.M., and Schellekens, H.

Published
2013

15. Knockdown of the glucocorticoid receptor alters functional integration of newborn neurons in the adult hippocampus and impairs fear-motivated behavior.

Author

Fitzsimons, C.P., Van Hooijdonk, L.W.A., Schouten, M., Zalachoras, I., Brinks, V., Zheng, T., Schouten, T.G., Saaltink, D.J., Dijkmans, T., Steindler, D.A., Verhaagen, J., Verbeek, F.J., Lucassen, P.J., De Kloet, E.R., Meijer, O.C., Karst, H., Joels, M., Oitzl, M.S., Vreugdenhil, E., Fitzsimons, C.P., Van Hooijdonk, L.W.A., Schouten, M., Zalachoras, I., Brinks, V., Zheng, T., Schouten, T.G., Saaltink, D.J., Dijkmans, T., Steindler, D.A., Verhaagen, J., Verbeek, F.J., Lucassen, P.J., De Kloet, E.R., Meijer, O.C., Karst, H., Joels, M., Oitzl, M.S., and Vreugdenhil, E.

Published
2013

16. Quality of Original and Biosimilar Epoetin Products

Author

Advanced drug delivery systems/drug targeting, Biomolecular Analysis, Innovation Studies, Farmaceutische Analyse, Pharmaceutics, Sub Biotechnological drugs, Sub Biomolecular analysis, Dep Farmaceutische wetenschappen, Brinks, V., Hawe, A., Basmeleh, A.H.H., Joachin-Rodriguez, L., Haselberg, R., Somsen, G.W., Jiskoot, W., Schellekens, H., Advanced drug delivery systems/drug targeting, Biomolecular Analysis, Innovation Studies, Farmaceutische Analyse, Pharmaceutics, Sub Biotechnological drugs, Sub Biomolecular analysis, Dep Farmaceutische wetenschappen, Brinks, V., Hawe, A., Basmeleh, A.H.H., Joachin-Rodriguez, L., Haselberg, R., Somsen, G.W., Jiskoot, W., and Schellekens, H.

Published
2011

17. Immunological mechanism underlying the immune response to tecombinant human protein therapeutics

Author

Advanced drug delivery systems/drug targeting, Innovation Studies, Pharmaceutics, Dep Farmaceutische wetenschappen, Section Innovation Studies, Sauerborn, M.S., Brinks, V., Jiskoot, W., Schellekens, H., Advanced drug delivery systems/drug targeting, Innovation Studies, Pharmaceutics, Dep Farmaceutische wetenschappen, Section Innovation Studies, Sauerborn, M.S., Brinks, V., Jiskoot, W., and Schellekens, H.

Published
2010

18. Hybrid transgenic immune tolerant mouse model for assessing the breaking of B cell tolerance by human interferon beta

Author

Advanced drug delivery systems/drug targeting, Innovation Studies, Pharmaceutics, Dep Farmaceutische wetenschappen, Sub Biotechnological drugs, Section Innovation Studies, van Beers, M.M.C., Sauerborn, M.S., Gili, F., Hermeling, S., Brinks, V., Schellekens, H., Jiskoot, W., Advanced drug delivery systems/drug targeting, Innovation Studies, Pharmaceutics, Dep Farmaceutische wetenschappen, Sub Biotechnological drugs, Section Innovation Studies, van Beers, M.M.C., Sauerborn, M.S., Gili, F., Hermeling, S., Brinks, V., Schellekens, H., and Jiskoot, W.

Published
2010

19. Knockdown of the glucocorticoid receptor alters functional integration of newborn neurons in the adult hippocampus and impairs fear-motivated behavior

Author

Fitzsimons, C P, primary, van Hooijdonk, L W A, additional, Schouten, M, additional, Zalachoras, I, additional, Brinks, V, additional, Zheng, T, additional, Schouten, T G, additional, Saaltink, D J, additional, Dijkmans, T, additional, Steindler, D A, additional, Verhaagen, J, additional, Verbeek, F J, additional, Lucassen, P J, additional, de Kloet, E R, additional, Meijer, O C, additional, Karst, H, additional, Joels, M, additional, Oitzl, M S, additional, and Vreugdenhil, E, additional

Published
2012
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20. From Corona Virus to Corona Crisis: The Value of An Analytical and Geographical Understanding of Crisis.

Author

Brinks V and Ibert O

Abstract

The term 'crisis' is omnipresent. The current corona virus pandemic is perceived as the most recent example. However, the notion of crisis is increasingly deployed as a signifier of relevance, rather than as an analytical concept. Moreover, human geography has so far little contributed to the interdisciplinary crisis research field which is fixated on the temporal aspects of crisis but neglects its spatiality. Against this background, the first aim of the paper is to demonstrate the value of thinking about crisis analytically. Therefore, we introduce theoretical knowledge developed within a recently emerging literature on crisis management. Second, we demonstrate the relevance of including geographical thinking into crisis research more systematically. Based on the TPSN-framework by Jessop et al ., we illustrate spatial dimensions of the 'corona crisis', its perception and handling in Germany. The empirical references are based on media reports., (© 2020 The Authors. Tijdschrift voor Economische en Sociale Geografie published by John Wiley & Sons Ltd on behalf of Royal Dutch Geographical Society / Koninklijk Nederlands Aardrijkskundig.)

Published
2020
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21. The Cystic Fibrosis-Like Airway Surface Layer Is not a Significant Barrier for Delivery of Eluforsen to Airway Epithelial Cells.

Author

Brinks V, Lipinska K, de Jager M, Beumer W, Button B, Livraghi-Butrico A, Henig N, and Matthee B

Subjects
Administration, Inhalation, Animals, Biofilms, Cells, Cultured, Cystic Fibrosis genetics, Epithelial Cells metabolism, Female, Humans, Male, Mice, Mice, Inbred C57BL, Oligonucleotides administration & dosage, Oligonucleotides pharmacokinetics, Oligonucleotides, Antisense administration & dosage, Oligonucleotides, Antisense pharmacokinetics, Pseudomonas aeruginosa physiology, Time Factors, Tissue Distribution, Cystic Fibrosis therapy, Cystic Fibrosis Transmembrane Conductance Regulator metabolism, Lung metabolism, Oligonucleotides pharmacology, Oligonucleotides, Antisense pharmacology
Abstract

Background: Eluforsen (previously known as QR-010) is a 33-mer antisense oligonucleotide under development for oral inhalation in cystic fibrosis (CF) patients with the delta F508 mutation. Previous work has shown that eluforsen restores CF transmembrane conductance regulator (CFTR) function in vitro and in vivo . To be effective, eluforsen has first to reach its primary target, the lung epithelial cells. Therefore, it has to diffuse through the CF airway surface layer (ASL), which in CF is characterized by the presence of thick and viscous mucus, impaired mucociliary clearance, and persistent infections. The goal of this study was to assess delivery of eluforsen through CF-like ASL. Methods and Results: First, air-liquid interface studies with cultured primary airway epithelial cells revealed that eluforsen rapidly diffuses through CF-like mucus at clinically relevant doses when nebulized once or repeatedly, over a range of testing doses. Furthermore, eluforsen concentrations remained stable in CF patient sputum for at least 48 hours, and eluforsen remained intact in the presence of various inhaled CF medications for at least 24 hours. When testing biodistribution of eluforsen after orotracheal administration in vivo , no differences in lung, liver, trachea, and kidney eluforsen concentration were observed between mice with a CF-like lung phenotype (ENaC-overexpressing mice) and control wild-type (WT) littermates. Also, eluforsen was visualized in the airway epithelial cell layer of CF-like muco-obstructed mice and WT littermates. Finally, studies of eluforsen uptake and binding to bacteria prevalent in CF lungs, and diffusion through bacterial biofilms showed that eluforsen was stable and not absorbed by, or bound to bacteria. In addition, eluforsen was found to be able to penetrate Pseudomonas aeruginosa biofilms. Conclusions: The thickened and concentrated CF ASL does not constitute a significant barrier for delivery of eluforsen, and feasibility of oral inhalation of eluforsen is supported by these data.

Published
2019
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22. Evaluation of the suitability of a Sprague Dawley rat model to assess intravenous iron preparations.

Author

Span K, Pieters EHE, Brinks V, Hennink WE, and Schellekens H

Subjects
Animals, Colloids administration & dosage, Colloids toxicity, Ferric Compounds administration & dosage, Ferric Compounds toxicity, Ferric Oxide, Saccharated, Glucaric Acid administration & dosage, Glucaric Acid toxicity, Hematinics administration & dosage, Infusions, Intravenous, Injections, Intravenous, Male, Nanoparticles administration & dosage, Nanoparticles toxicity, Rats, Sprague-Dawley, Reproducibility of Results, Hematinics toxicity, Kidney drug effects, Liver drug effects, Models, Animal, Rats
Abstract

The aim of the study was to examine the reproducibility of a rat model to assess the preclinical similarity in safety profiles and tissue accumulation of iron products. Accordingly, the effect of several doses of intravenously administered Venofer® and of Ferrlecit® on blood parameters, and on kidney and particularly liver toxicity were examined in non-anemic Sprague Dawley rats. The different analysis showed neither a clear treatment nor a dose effect after multiple injections. The parameters measured in this rat strain showed some iron induced adverse effects, but these could not be correlated to treatment specific differences. The findings presented in this paper indicate the difficulty to define a useful preclinical model to evaluate iron-based nano-colloidal preparations., (Copyright © 2017 Elsevier Inc. All rights reserved.)

Published
2018
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23. The Use of Magnetic Resonance Imaging for Non-Invasive Assessment of Venofer® Biodistribution in Rats.

Author

Span K, Pieters EHE, Hennink WE, van der Toorn A, Brinks V, Dijkhuizen RM, and van Tilborg GAF

Subjects
Animals, Drug Evaluation, Preclinical methods, Ferric Oxide, Saccharated administration & dosage, Half-Life, Hematinics administration & dosage, Injections, Intravenous, Kidney diagnostic imaging, Kidney metabolism, Liver diagnostic imaging, Liver metabolism, Male, Models, Animal, Rats, Rats, Sprague-Dawley, Spleen diagnostic imaging, Spleen metabolism, Tissue Distribution, Ferric Oxide, Saccharated pharmacokinetics, Hematinics pharmacokinetics, Magnetic Resonance Imaging, Whole Body Imaging
Abstract

Purpose: The aim of this study was to determine the potential of magnetic resonance imaging to evaluate the biodistribution of exogenous iron within 24 h after one single injection of Venofer® (iron sucrose)., Methods: Venofer® was evaluated in vitro for its ability to generate contrast in MR images. Subsequently, iron disposition was assessed in rats with MRI, in vivo up to 3 h and post mortem at 24 h after injection of Venofer®, at doses of 10- and 40 mg/kg body weight (n = 2 × 4), or saline (n = 4)., Results: Within 10-20 min after injection of Venofer®, transverse relaxation rates (R 2 ) clearly increased, representative of a local increase in iron concentration, in liver, spleen and kidney, including the kidney medulla and cortex. In liver and spleen R 2 values remained elevated up to 3 h post injection, while the initial R 2 increase in the kidney was followed by gradual decrease towards baseline levels. Bone marrow and muscle tissue did not show significant increases in R 2 values. Whole-body post mortem MRI showed most prominent iron accumulation in the liver and spleen at 24 h post injection, which corroborated the in vivo results., Conclusions: MR imaging is a powerful imaging modality for non-invasive assessment of iron distribution in organs. It is recommended to use this whole-body imaging approach complementary to other techniques that allow quantification of iron disposition at a (sub)cellular level.

Published
2018
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24. A novel oral iron-complex formulation: Encapsulation of hemin in polymeric micelles and its in vitro absorption.

Author

Span K, Verhoef JJF, Hunt H, van Nostrum CF, Brinks V, Schellekens H, and Hennink WE

Subjects
Acrylamides chemistry, Anemia blood, Ascorbic Acid chemistry, Caco-2 Cells, Cell Survival, Drug Delivery Systems, Ferric Compounds chemistry, Ferritins chemistry, Heme chemistry, Humans, Hydrogen-Ion Concentration, Iron chemistry, Micelles, Microscopy, Confocal, Molecular Weight, Particle Size, Polyethylene Glycols chemistry, Sulfates chemistry, Temperature, Ultraviolet Rays, Administration, Oral, Drug Carriers chemistry, Hemin chemistry, Polymers chemistry
Abstract

Anemia resulting from iron deficiency is one of the most prevalent diseases in the world. As iron has important roles in several biological processes such as oxygen transport, DNA synthesis and cell growth, there is a high need for iron therapies that result in high iron bioavailability with minimal toxic effects to treat patients suffering from anemia. This study aims to develop a novel oral iron-complex formulation based on hemin-loaded polymeric micelles composed of the biodegradable and thermosensitive polymer methoxy-poly(ethylene glycol)-b-poly[N-(2-hydroxypropyl)methacrylamide-dilactate], abbreviated as mPEG-b-p(HPMAm-Lac 2 ). Hemin-loaded micelles were prepared by addition of hemin dissolved in DMSO:DMF (1:9, one volume) to an aqueous polymer solution (nine volumes) of mPEG-b-p(HPMAm-Lac 2 ) followed by rapidly heating the mixture at 50°C to form hemin-loaded micelles that remain intact at room and physiological temperature. The highest loading capacity for hemin in mPEG-b-p(HPMAm-Lac 2 ) micelles was 3.9%. The average particle diameter of the hemin-micelles ranged from 75 to 140nm, depending on the concentration of hemin solution that was used to prepare the micelles. The hemin-loaded micelles were stable at pH 2 for at least 3 h which covers the residence time of the formulation in the stomach after oral administration and up to 17 h at pH 7.4 which is sufficient time for uptake of the micelles by the enterocytes. Importantly, incubation of Caco-2 cells with hemin-micelles for 24 h at 37°C resulted in ferritin levels of 2500ng/mg protein which is about 10-fold higher than levels observed in cells incubated with iron sulfate under the same conditions. The hemin formulation also demonstrated superior cell viability compared to iron sulfate with and without ascorbic acid. The study presented here demonstrates the development of a promising novel iron complex for oral delivery., (Copyright © 2016 Elsevier B.V. All rights reserved.)

Published
2016
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25. Quality and Batch-to-Batch Consistency of Original and Biosimilar Epoetin Products.

Author

Halim LA, Brinks V, Jiskoot W, Romeijn S, Haselberg R, Burns C, Wadhwa M, and Schellekens H

Subjects
Animals, Biosimilar Pharmaceuticals analysis, Biosimilar Pharmaceuticals chemistry, Epoetin Alfa analysis, Epoetin Alfa chemistry, Erythropoietin analysis, Erythropoietin chemistry, Female, Humans, Mice, Mice, Inbred BALB C, Recombinant Proteins analysis, Recombinant Proteins chemistry, Recombinant Proteins standards, Therapeutic Equivalency, Biosimilar Pharmaceuticals standards, Chemistry, Pharmaceutical methods, Epoetin Alfa standards, Erythropoietin standards
Abstract

Comprehensive physicochemical characterization and biological assays are essential parts in assessing quality attributes of biologicals. Here, we compared the quality of different marketed recombinant human erythropoietin (epoetin) products: originators, Eprex and NeoRecormon as well as 2 biosimilars, Retacrit and Binocrit. In addition, assessment of batch-to-batch variability was included by collecting 2 or more batches of each product. Common assays which included sodium dodecyl sulfate-polyacrylamide gel electrophoresis, high-performance size-exclusion chromatography, asymmetrical flow field-flow fractionation, capillary zone electrophoresis, and potency testing were used. Of the tested products and among batches of single products, variations in epoetin content, isoform profiles, and potency were found. Ultimately, this study demonstrated the high quality of epoetin products with some degree of variation among products and batches, confirming the "similar but not identical" paradigm of biologicals., (Copyright © 2016. Published by Elsevier Inc.)

Published
2016
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26. Development of ADA against recombinant human interferon beta in immune tolerant mice requires rapid recruitment of CD4⁺ T cells, induces formation of germinal centers but lacks susceptibility for (most) adjuvants.

Author

Kijanka G, Sauerborn M, Boon L, Schellekens H, and Brinks V

Subjects
Animals, Antibodies administration & dosage, CD4-Positive T-Lymphocytes cytology, Germinal Center cytology, Humans, Interferon-beta administration & dosage, Mice, Mice, Inbred C57BL, Mice, Transgenic, Recombinant Proteins administration & dosage, Recombinant Proteins immunology, Adjuvants, Immunologic, Antibodies immunology, CD4-Positive T-Lymphocytes immunology, Germinal Center immunology, Immune Tolerance, Interferon-beta immunology
Abstract

Immunological processes leading to formation of antidrug antibodies (Abs) against recombinant human proteins remain poorly understood. Animal and clinical studies revealed that immunogenicity shares both T-cell-dependent (requirement of CD4(+) T cells, isotype switching) and T-cell-independent (involvement of Marginal Zone B cells, apparent lack of memory) characteristics. We used immune tolerant mice to study the mechanism underlying immunogenicity in more detail. We found that CD4(+) T cells were crucial at early stages of Ab responses against rhIFNβ. In addition, we found a similar number of germinal centers (GCs) in spleen after rhIFNβ treatment as after treatment with a foreign protein. However, neither Ab titers nor the number of GCs was increased by adsorption of rhIFNβ on aluminum hydroxide. Therefore, we tested the effect of several immune adjuvants in a follow-up study. We found that only conjugation of rhIFNβ to a carrier protein (cholera toxin subunit B) was effective in boosting Ab titers. However, these conjugates failed to trigger rhIFNβ specific memory formation. Our findings show that early events of the immunogenicity reaction to self-proteins are CD4(+) T-cell dependent. Nevertheless, despite those similarities, immunogenicity of human proteins is clearly not a classical CD4(+) T-cell-dependent response., (© 2014 Wiley Periodicals, Inc. and the American Pharmacists Association.)

Published
2015
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27. A modified immune tolerant mouse model to study the immunogenicity of recombinant human interferon beta.

Author

Abdolvahab MH, Brinks V, and Schellekens H

Subjects
Animals, Crosses, Genetic, Disease Models, Animal, Female, Humans, Interferon-beta administration & dosage, Male, Mice, Mice, Inbred C57BL, Mice, Transgenic, Multiple Sclerosis blood, Multiple Sclerosis immunology, Multiple Sclerosis pathology, Recombinant Proteins administration & dosage, Species Specificity, Antibodies blood, Immune Tolerance, Interferon-beta immunology, Recombinant Proteins immunology
Abstract

Interferon beta may induce antibodies in multiple sclerosis patients and the incidence of immunogenicity depends on the type of product. These antibodies can reduce the efficacy of interferon beta. Two transgenic immune tolerant mouse models for human interferon beta (hIFNβ) (C57Bl/6, and C57Bl/6×FVB/N F1 hybrid mice) have been developed previously for studying immunogenicity. These models, however, may not be used for every interferon beta product because of the lack of immunogenicity in the wildtype genetic background. We therefore developed a modified transgenic mouse model by backcrossing the F1 hybrid C57Bl/6×FVB/N transgenic mice with wildtype FVB/N for 10 generations. These F10 offspring (referred to hear as FVB/N) have a genetic background consisting of mostly FVB/N (99.9%) and very little C57Bl/6 (0.1%), and are expected to have the more sensitive antibody producing phenotype of the parental FVB/N strain. The newly generated "FVB/N" strain was assessed for antibody formation against different rhIFNβ formulations compared to the C57Bl/6, and C57Bl/6×FVB/N transgenic mouse models. The new FVB/N transgenic mouse model was more sensitive for all tested rhIFNβ products, and the difference in antibody titers between the transgenic and non-transgenic mice of the FVB/N strain was much bigger compared to the antibody levels of the C57Bl/6, and C57Bl/6×FVB/N strains., (Copyright © 2014 Elsevier B.V. All rights reserved.)

Published
2014
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28. The effects of dodecyl maltoside and sodium dodecyl sulfate surfactants on the stability and aggregation of recombinant interferon Beta-1b.

Author

Haji Abdolvahab M, Fazeli A, Fazeli MR, Brinks V, and Schellekens H

Subjects
Antiviral Agents pharmacology, Cell Line, Tumor, Humans, Hydrophobic and Hydrophilic Interactions, Interferon beta-1b, Interferon-beta pharmacology, Protein Multimerization, Protein Stability, Recombinant Proteins pharmacology, Sodium Dodecyl Sulfate chemistry, Solubility, Antiviral Agents chemistry, Glucosides chemistry, Interferon-beta chemistry, Recombinant Proteins chemistry
Abstract

Aggregation often occurs during manufacturing and storage of protein drugs. Detergents such as sodium dodecyl sulfate are commonly used to prevent aggregation but need to be eliminated before final formulation for safety reasons. We studied the ability of dodecylmaltoside (DDM), a nontoxic alkyl saccharide surfactant, to reduce aggregation and increase the stability of interferon beta-1b (IFN)-β-1b. An increase of 8°C in the Tm of IFN-β-1b was observed when 0.1% of DDM was present in the protein solution. The absorption of DDM on hydrophobic surfaces of IFN-β-1b enables the surface to become hydrophilic and non-ionic, and increases the stability of the protein. 0.1% DDM also results in a 62% increase in helical and a 25% decrease in β-sheet structures. 0.1% DDM not only suppresses aggregate formation but also improves IFN-β-1b solubilization. Furthermore, we have showed the protective effect of DDM on the anti-viral activity of IFN-β-1b in solution.

Published
2014
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29. Development of a transgenic mouse model to study the immunogenicity of recombinant human insulin.

Author

Torosantucci R, Brinks V, Kijanka G, Halim LA, Sauerborn M, Schellekens H, and Jiskoot W

Subjects
Animals, Chemistry, Pharmaceutical methods, Humans, Immune Tolerance immunology, Insulin chemistry, Mice, Mice, Inbred BALB C, Nanoparticles chemistry, Particle Size, Polystyrenes chemistry, Recombinant Proteins chemistry, Antibody Formation immunology, Insulin immunology, Mice, Transgenic immunology, Recombinant Proteins immunology
Abstract

Mouse models are commonly used to assess the immunogenicity of therapeutic proteins and to investigate the immunological processes leading to antidrug antibodies. The aim of this work was to develop a transgenic (TG) Balb/c mouse model for evaluating the immunogenicity of recombinant human insulin (insulin) formulations. Validation of the model was performed by measuring the antibody response against plain and particulate insulin in TG and nontransgenic (NTG) mice. Intraperitoneal administration of insulin (20 μg/dose, 12 doses over a period of 4 weeks) did not break the immune tolerance of the TG mice, whereas it did elicit antibodies in NTG mice. The immune tolerance of TG mice could be circumvented, albeit at low titers, by administering insulin covalently bound to 50-nm polystyrene nanoparticles. The TG mouse model was employed to compare the immunogenicity of oxidized aggregated insulin, oxidized nonaggregated insulin, and three commercially available formulations of insulin variants (i.e., Levemir®, Insulatard®, and Actrapid®). Oxidized insulin, aggregated or nonaggregated, was moderately immunogenic in TG mice (50% and 33% responders, respectively), whereas the immunogenicity of the commercial formulations was low. This model can be used to compare the immunogenicity of insulin formulations and to study immune mechanisms of antibody formation against insulin., (© 2014 Wiley Periodicals, Inc. and the American Pharmacists Association.)

Published
2014
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30. How bio-questionable are the different recombinant human erythropoietin copy products in Thailand?

Author

Halim LA, Brinks V, Jiskoot W, Romeijn S, Praditpornsilpa K, Assawamakin A, and Schellekens H

Subjects
Blotting, Western, Chromatography, Gel, Chromatography, High Pressure Liquid, Electrophoresis, Polyacrylamide Gel, Erythropoietin isolation & purification, Fractionation, Field Flow, Humans, Recombinant Proteins isolation & purification, Recombinant Proteins pharmacology, Thailand, Erythropoietin pharmacology
Abstract

Purpose: The high prevalence of pure red cell aplasia in Thailand has been associated with the sharp increase in number of recombinant human erythropoietin (rhEPO) copy products, based on a classical generic regulatory pathway, which have entered the market. This study aims to assess the quality of rhEPO copy products being used in Thailand., Methods: Twelve rhEPO copy products were purchased from pharmacies in Thailand, shipped under controlled cold chain conditions to the Netherlands and characterized using (1) high performance size-exclusion chromatography, (2) asymmetrical flow field-flow fractionation, (3) sodium dodecyl sulfate polyacrylamide gel electrophoresis in combination with (4) Western blotting and additionally tested for (5) host cell protein impurities as well as (6) endotoxin contamination., Results: Some of the tested rhEPO copy products showed high aggregate levels and contained a substantial amount of protein fragments. Also, one of rhEPO copy products had a high endotoxin level, exceeding the FDA limit., Conclusions: Our observations show that some of the tested copy products on the Thai market differ significantly from the originator rhEPO product, Epogen®. This comparison study supports a link between the quality attributes of copy rhEPO products and their immunogenicity.

Published
2014
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31. Influence of aggregation and route of injection on the biodistribution of mouse serum albumin.

Author

Kijanka G, Prokopowicz M, Schellekens H, and Brinks V

Subjects
Animals, Electrophoresis, Polyacrylamide Gel, Female, Fluorescent Dyes administration & dosage, Fluorescent Dyes chemistry, Fluorescent Dyes pharmacokinetics, Injections, Intramuscular, Injections, Intraperitoneal, Injections, Intravenous, Injections, Subcutaneous, Luminescent Measurements methods, Mice, Serum Albumin chemistry, Tissue Distribution, Liver metabolism, Lung metabolism, Serum Albumin administration & dosage, Serum Albumin pharmacokinetics, Spleen metabolism
Abstract

Protein aggregates are a major risk factor for immunogenicity. Until now most studies on aggregate-driven immunogenicity have focused on linking physicochemical features of the aggregates to the formation of anti-drug antibodies. Lacking is however, basic knowledge on the effect of aggregation on the biodistribution and clearance of therapeutic proteins in vivo. The aim of current study was to get insight into the effect of aggregation on biodistribution in mice using different routes of administration. Fluorescently labeled stressed and unstressed mouse serum albumin was injected via different routes in mice and detected via in vivo fluorescence imaging up to 48 hrs post-injection. We found that biodistribution of stressed MSA significantly differed from its unstressed counterpart. Subcutaneous and intramuscular administration resulted in accumulation of protein at the site of injection, from which clearance of stressed MSA was considerably slower than clearance of unstressed MSA. Upon intravenous and intraperitoneal injection of stressed MSA, fluorescent "hotspots" were observed in the spleens, livers and lungs. Further and more detailed examination of biodistribution after intraperitoneal injection showed higher fluorescence in most of tested organs suggesting more efficient diffusion and/or lymphatic uptake from peritoneum of unstressed MSA than the stressed formulation.

Published
2014
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32. Immunogenicity of mAbs in non-human primates during nonclinical safety assessment.

Author

van Meer PJ, Kooijman M, Brinks V, Gispen-de Wied CC, Silva-Lima B, Moors EH, and Schellekens H

Subjects
Animals, Antibodies, Monoclonal adverse effects, Drug Approval statistics & numerical data, Drug Evaluation, Preclinical methods, Drug Evaluation, Preclinical statistics & numerical data, Drug Industry statistics & numerical data, Drug-Related Side Effects and Adverse Reactions etiology, European Union, Humans, Mice, Registries statistics & numerical data, Antibodies, Monoclonal immunology, Antibody Formation immunology, Drug-Related Side Effects and Adverse Reactions immunology, Primates immunology
Abstract

The immunogenicity of biopharmaceuticals used in clinical practice remains an unsolved challenge in drug development. Non-human primates (NHPs) are often the only relevant animal model for the development of monoclonal antibodies (mAbs), but the immune response of NHPs to therapeutic mAbs is not considered to be predictive of the response in humans because of species differences. In this study, we accessed the drug registration files of all mAbs registered in the European Union to establish the relative immunogenicity of mAbs in NHPs and humans. The incidence of formation of antidrug-antibodies in NHPs and patients was comparable in only 59% of the cases. In addition, the type of antidrug-antibody response was different in NHP and humans in 59% of the cases. Humanization did not necessarily reduce immunogenicity in humans. Immunogenicity interfered with the safety assessment during non-clinical drug development when clearing or neutralizing antibodies were formed. While important to interpret the study results, immunogenicity reduced the quality of NHP data in safety assessment. These findings confirm that the ability to compare relative immunogenicity of mAbs in NHPs and humans is low. Furthermore, immunogenicity limits the value of informative NHP studies.

Published
2013
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33. The immunogenicity of polyethylene glycol: facts and fiction.

Author

Schellekens H, Hennink WE, and Brinks V

Subjects
Animals, Antibody Formation, Drug Delivery Systems methods, Humans, Liposomes chemistry, Liposomes immunology, Polyethylene Glycols chemistry, Proteins chemistry, Antibodies immunology, Polyethylene Glycols metabolism, Proteins immunology, Proteins therapeutic use
Abstract

An increasing number of pegylated therapeutic proteins and drug targeting compounds are being introduced in the clinic. Pegylation is intended to increase circulation time and to reduce an immunogenic response. Recently however a number of publications have appeared claiming that the polyethylene glycol (PEG) moiety of these products in itself may be immunogenic and that the induced anti-PEG antibodies are linked to enhanced blood clearance and reduced efficacy of the products. A critical review of the literature shows that most, if not all assays for anti-PEG antibodies are flawed and lack specificity. Also the biological effects induced by anti-PEG antibodies lack the characteristics of a bona fide antibody reaction. Standardization of the anti-PEG assays and the development of reference sera are urgently needed.

Published
2013
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34. Preclinical models used for immunogenicity prediction of therapeutic proteins.

Author

Brinks V, Weinbuch D, Baker M, Dean Y, Stas P, Kostense S, Rup B, and Jiskoot W

Subjects
Animals, Computer Simulation, Humans, Immune System drug effects, Lymphocyte Activation drug effects, Models, Biological, Drug Evaluation, Preclinical methods, Proteins immunology, Proteins therapeutic use
Abstract

All therapeutic proteins are potentially immunogenic. Antibodies formed against these drugs can decrease efficacy, leading to drastically increased therapeutic costs and in rare cases to serious and sometimes life threatening side-effects. Many efforts are therefore undertaken to develop therapeutic proteins with minimal immunogenicity. For this, immunogenicity prediction of candidate drugs during early drug development is essential. Several in silico, in vitro and in vivo models are used to predict immunogenicity of drug leads, to modify potentially immunogenic properties and to continue development of drug candidates with expected low immunogenicity. Despite the extensive use of these predictive models, their actual predictive value varies. Important reasons for this uncertainty are the limited/insufficient knowledge on the immune mechanisms underlying immunogenicity of therapeutic proteins, the fact that different predictive models explore different components of the immune system and the lack of an integrated clinical validation. In this review, we discuss the predictive models in use, summarize aspects of immunogenicity that these models predict and explore the merits and the limitations of each of the models.

Published
2013
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35. Identification of oxidation sites and covalent cross-links in metal catalyzed oxidized interferon Beta-1a: potential implications for protein aggregation and immunogenicity.

Author

Torosantucci R, Sharov VS, van Beers M, Brinks V, Schöneich C, and Jiskoot W

Subjects
Ascorbic Acid chemistry, Benzene Derivatives chemistry, Chromatography, Gel, Circular Dichroism, Copper chemistry, Humans, Interferon-beta immunology, Methylamines chemistry, Molecular Structure, Spectrometry, Fluorescence, Spectrometry, Mass, Electrospray Ionization, Tandem Mass Spectrometry, Interferon-beta chemistry
Abstract

Oxidation via Cu(2+)/ascorbate of recombinant human interferon beta-1a (IFNβ1a) leads to highly immunogenic aggregates, however it is unknown which amino acids are modified and how covalent aggregates are formed. In the present work we mapped oxidized and cross-linked amino acid residues in aggregated IFNβ1a, formed via Cu(2+)/ascorbate catalyzed oxidation. Size exclusion chromatography (SEC) was used to confirm extensive aggregation of oxidized IFNβ1a. Circular dichroism and intrinsic fluorescence spectroscopy indicated substantial loss of secondary and tertiary structure, respectively. Derivatization with 4-(aminomethyl)benzenesulfonic acid was used to demonstrate, by fluorescence in combination with SEC, the presence of tyrosine (Tyr) oxidation products. High performance liquid chromatography coupled to electrospray ionization mass spectrometry of reduced, alkylated, and digested protein was employed to localize chemical degradation products. Oxidation products of methionine, histidine, phenylalanine (Phe), tryptophan, and Tyr residues were identified throughout the primary sequence. Covalent cross-links via 1,4- or 1,6-type addition between primary amines and DOCH (2-amino-3-(3,4-dioxocyclohexa-1,5-dien-1-yl)propanoic acid, an oxidation product of Phe and Tyr) were detected. There was no evidence of disulfide bridge, Schiff base, or dityrosine formation. The chemical cross-links identified in this work are most likely responsible for the formation of covalent aggregates of IFNβ1a induced by oxidation, which have previously been shown to be highly immunogenic.

Published
2013
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36. Effect of treatment regimen on the immunogenicity of human interferon Beta in immune tolerant mice.

Author

Kijanka G, Jiskoot W, Schellekens H, and Brinks V

Subjects
Animals, Antibody Formation, Drug Administration Routes, Humans, Immune Tolerance, Mice, Transgenic, Multiple Sclerosis drug therapy, Multiple Sclerosis immunology, Antibodies immunology, Interferon-beta administration & dosage, Interferon-beta immunology
Abstract

Purpose: Interferon beta is commonly used as therapeutic in the first line of therapy for multiple sclerosis. However, depending on the product, it induces an antibody response in up to 60% of patients. This study evaluated the impact of therapy related factors like dose, route of administration and administration frequency on the immunogenicity of one of the originator interferon beta drugs (Betaferon®) in an immune tolerant transgenic mouse model., Methods: Immune tolerant transgenic mice received injections with Betaferon® via different routes, doses and injection frequencies. Anti-drug antibody (ADA) production was measured by ELISA to assess immunogenicity., Results: A single injection of Betaferon® was found to be sufficient for the induction of ADAs. The antibody titer was enhanced with increasing dose and treatment frequency. Among the tested administration routes, the intravenous route was the most immunogenic one, which is in contradiction with one of the dogma in immunogenicity research according to which subcutaneous administration is the most immunogenic route. Intramuscular, intraperitoneal and subcutaneous injections resulted in comparable immunogenicity., Conclusion: This study shows that treatment related factors affect significantly immunogenicity of Betaseron® and therefore substantiate the need for further studies on these factors in patients.

Published
2013
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37. Antibody response against Betaferon® in immune tolerant mice: involvement of marginal zone B-cells and CD4+ T-cells and apparent lack of immunological memory.

Author

Sauerborn M, van Beers MM, Jiskoot W, Kijanka GM, Boon L, Schellekens H, and Brinks V

Subjects
Animals, B-Lymphocyte Subsets classification, B-Lymphocyte Subsets drug effects, CD4-Positive T-Lymphocytes drug effects, Female, Interferon beta-1b, Interferon-beta administration & dosage, Lymphocyte Cooperation drug effects, Lymphocyte Cooperation immunology, Lymphocyte Depletion, Lymphoid Tissue cytology, Lymphoid Tissue drug effects, Male, Mice, Mice, Inbred C57BL, Mice, Transgenic, Models, Animal, Recombinant Proteins administration & dosage, Recombinant Proteins antagonists & inhibitors, Recombinant Proteins immunology, B-Lymphocyte Subsets immunology, CD4-Positive T-Lymphocytes immunology, Immune Tolerance drug effects, Immunoglobulin G biosynthesis, Immunologic Memory drug effects, Interferon-beta antagonists & inhibitors, Interferon-beta immunology, Lymphoid Tissue immunology
Abstract

Purpose: The immunological processes underlying immunogenicity of recombinant human therapeutics are poorly understood. Using an immune tolerant mouse model we previously demonstrated that aggregates are a major trigger of the antidrug antibody (ADA) response against recombinant human interferon beta (rhIFNβ) products including Betaferon®, and that immunological memory seems to be lacking after a rechallenge with non-aggregated rhIFNβ. The apparent absence of immunological memory indicates a CD4+ T-cell independent (Tind) immune response underlying ADA formation against Betaferon®. This hypothesis was tested., Methods: Using the immune tolerant mouse model we first validated that rechallenge with highly aggregated rhIFNβ (Betaferon®) does not lead to a subsequent fast increase in ADA titers, suggesting a lack of immunological memory. Next we assessed whether Betaferon® could act as Tind antigen by inactivation of marginal zone (MZ) B-cells during treatment. MZ B-cells are major effector cells involved in a Tind immune response. In a following experiment we depleted the mice from CD4+ T-cells to test their involvement in the ADA response against Betaferon®., Results: Inactivation of MZ B-cells at the start of Betaferon® treatment drastically lowered ADA levels, suggesting a Tind immune response. However, persistent depletion of CD4+ T-cells before and during Betaferon® treatment abolished the ADA response in almost all mice., Conclusion: The immune response against rhIFNβ in immune tolerant mice is neither a T-cell independent nor a classical T-cell dependent immune response. Further studies are needed to confirm absence of immunological memory (cells).

Published
2013
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38. Immunogenicity of different stressed IgG monoclonal antibody formulations in immune tolerant transgenic mice.

Author

Filipe V, Jiskoot W, Basmeleh AH, Halim A, Schellekens H, and Brinks V

Subjects
Animals, Antibody Formation, Epitopes immunology, Humans, Immune Tolerance, Immunoglobulin G genetics, Immunoglobulin G immunology, Immunoglobulin Heavy Chains genetics, Immunoglobulin Light Chains genetics, Mice, Mice, Transgenic, Protein Conformation, Protein Multimerization immunology, Immunoglobulin G metabolism, Pharmaceutical Preparations metabolism
Abstract

The presence of protein aggregates in biopharmaceutical formulations is of great concern for safety and efficacy reasons. The aim of this study was to correlate the type and amount of IgG monoclonal antibody aggregates with their immunogenic potential. IgG degradation was obtained by freeze-thawing cycles, pH-shift cycles, heating, shaking and metal-catalyzed oxidation. The size, amount, morphology and type of intermolecular bonds of aggregates, as well as structural changes and epitope integrity were characterized. These formulations were injected in mice transgenic (TG) for human genes for Ig heavy and light chains and their non-transgenic (NTG) counterparts. Anti-drug antibody (ADA) titers were determined by bridging ELISA. Both unstressed IgG and freeze-thawed formulation did not induce measurable ADA levels. A mild antibody response was obtained in a fairly small percentage of mice, when injected with shaken, pH-shifted and heated formulations. The metal-catalyzed oxidized IgG formulation was the most immunogenic one, in both ADA titers and number of responders. The overall titers of NTG responders were significantly higher than the ones produced by TG mice, whereas there was no significant difference between the overall number of TG and NTG responders. This study reinforces the important role of protein aggregates on immunogenicity of therapeutic proteins and provides new insight into the immunogenic potential of different types of IgG aggregates. The results indicate that the quality of the IgG aggregates has more impact on the development of an immune response than their quantity or size.

Published
2012
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39. Immunogenicity of therapeutic proteins: the use of animal models.

Author

Brinks V, Jiskoot W, and Schellekens H

Subjects
Animals, Biological Products immunology, Biological Products pharmacology, Humans, Predictive Value of Tests, Drug Evaluation, Preclinical methods, Models, Animal, Proteins immunology, Proteins pharmacology
Abstract

Immunogenicity of therapeutic proteins lowers patient well-being and drastically increases therapeutic costs. Preventing immunogenicity is an important issue to consider when developing novel therapeutic proteins and applying them in the clinic. Animal models are increasingly used to study immunogenicity of therapeutic proteins. They are employed as predictive tools to assess different aspects of immunogenicity during drug development and have become vital in studying the mechanisms underlying immunogenicity of therapeutic proteins. However, the use of animal models needs critical evaluation. Because of species differences, predictive value of such models is limited, and mechanistic studies can be restricted. This review addresses the suitability of animal models for immunogenicity prediction and summarizes the insights in immunogenicity that they have given so far.

Published
2011
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40. Oxidized and aggregated recombinant human interferon beta is immunogenic in human interferon beta transgenic mice.

Author

van Beers MM, Sauerborn M, Gilli F, Brinks V, Schellekens H, and Jiskoot W

Subjects
Animals, Antibodies, Neutralizing immunology, Antibody Formation immunology, Chromatography, High Pressure Liquid methods, Guanidine chemistry, Humans, Hydrogen Peroxide chemistry, Immune Tolerance immunology, Interferon beta-1a, Interferon-beta pharmacology, Mice, Mice, Inbred C57BL, Mice, Transgenic, Oxidation-Reduction, Protein Binding immunology, Protein Folding, Protein Structure, Tertiary, Recombinant Proteins chemistry, Recombinant Proteins immunology, Recombinant Proteins pharmacology, Interferon-beta chemistry, Interferon-beta immunology
Abstract

Purpose: To study the effect of oxidation on the structure of recombinant human interferon beta-1a (rhIFNβ-1a) and its immunogenicity in wild-type and immune-tolerant transgenic mice., Methods: Untreated rhIFNβ-1a was degraded by metal-catalyzed oxidation, H(2)O(2)-mediated oxidation, and guanidine-mediated unfolding/refolding. Four rhIFNβ-1a preparations with different levels of oxidation and aggregation were injected intraperitoneally in mice 15× during 3 weeks. Both binding and neutralizing antibodies were measured., Results: All rhIFNβ-1a preparations contained substantial amounts of aggregates. Metal-catalyzed oxidized rhIFNβ-1a contained high levels of covalent aggregates as compared with untreated rhIFNβ-1a. H(2)O(2)-treated rhIFNβ-1a showed an increase in oligomer and unrecovered protein content by HP-SEC; RP-HPLC revealed protein oxidation. Guanidine-treated rhIFNβ-1a mostly consisted of dimers and oligomers and some non-covalent aggregates smaller in size than those in untreated rhIFNβ-1a. All degraded samples showed alterations in tertiary protein structure. Wild-type mice showed equally high antibody responses against all preparations. Transgenic mice were discriminative, showing elevated antibody responses against both metal-catalyzed oxidized and H(2)O(2)-treated rhIFNβ-1a as compared to untreated and guanidine-treated rhIFNβ-1a., Conclusions: Oxidation-mediated aggregation increased the immunogenicity of rhIFNβ-1a in transgenic mice, whereas aggregated preparations devoid of measurable oxidation levels were hardly immunogenic.

Published
2011
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41. Natural antibodies against bone morphogenic proteins and interferons in healthy donors and in patients with infections linked to type-1 cytokine responses.

Author

Sauerborn M, van de Vosse E, Delawi D, van Dissel JT, Brinks V, and Schellekens H

Subjects
Aged, Animals, Antigen-Antibody Reactions, CHO Cells, Cricetinae, Humans, Recombinant Proteins immunology, Recombinant Proteins therapeutic use, Autoantibodies blood, Autoantibodies immunology, Bone Morphogenetic Protein 2 immunology, Bone Morphogenetic Protein 7 immunology, Cytokines immunology, Interferons immunology
Abstract

In patients receiving recombinant therapeutic proteins, the production of antibodies against the therapeutics is a rising problem. The antibodies can neutralize and interfere with the efficacy and safety of drugs and even cause severe side effects if they cross-react against the natural, endogenous protein. Various factors have been identified to influence the immunogenic potential of recombinant human therapeutics, including several patients' characteristics. In recent years, so-called naturally occurring antibodies against cytokines and growth factors have been detected in naive patients before start of treatment with recombinant human therapeutics. The role of naturally occurring antibodies is not well understood and their influence on production of anti-drug antibodies is not known. One might speculate that the presence of naturally occurring antibodies increases the likelihood of eliciting anti-drug antibodies once treatment with the corresponding recombinant therapeutic protein is started. We screened serum samples from 410 healthy controls and patients for auto-antibodies against bone morphogenetic proteins (BMPs) 2 and 7 and interferon (IFN)-α, -β, and -γ in a new 3-step approach: rough initial screening, followed by competition and protein A/G depletion. Naturally occurring antibodies against these proteins were detected in 2% to 4% of the tested sera. Individuals who are 65 years or older had a slightly higher occurrence of naturally occurring antibodies. Auto-antibodies against BMP-7 and IFN-α were mainly comprised of IgM isotypes, and natural antibodies against BMP-2, IFN-β, and -γ were mainly IgG. To ensure assay specificity, assays were also used to detect antibodies against BMP-7 in patients being treated with rhBMP-7 before and after surgical procedure. Fifty percent of the treated patients had persistent anti-BMP-7 antibodies over time. The 3-step approach provides an attractive tool to identify naturally occurring antibodies in naive patients.

Published
2011
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42. Aggregated recombinant human interferon Beta induces antibodies but no memory in immune-tolerant transgenic mice.

Author

van Beers MM, Sauerborn M, Gilli F, Brinks V, Schellekens H, and Jiskoot W

Subjects
Animals, Binding Sites, Antibody, Blotting, Western, Chromatography, Gel, Electrophoresis, Polyacrylamide Gel, Enzyme-Linked Immunosorbent Assay, Humans, Interferon Type I genetics, Light, Mice, Mice, Transgenic, Recombinant Proteins, Scattering, Radiation, Spectrometry, Fluorescence, Antibodies, Neutralizing blood, Immune Tolerance genetics, Immunologic Memory genetics, Interferon Type I adverse effects, Interferon Type I immunology
Abstract

Purpose: To study the influence of protein aggregation on the immunogenicity of recombinant human interferon beta (rhIFNbeta) in wild-type mice and transgenic, immune-tolerant mice, and to evaluate the induction of immunological memory., Methods: RhIFNbeta-1b and three rhIFNbeta-1a preparations with different aggregate levels were injected intraperitoneally in mice 15x during 3 weeks, and the mice were rechallenged with rhIFNbeta-1a. The formation of binding (BABs) and neutralizing antibodies (NABs) was monitored., Results: Bulk rhIFNbeta-1a contained large, mainly non-covalent aggregates and stressed rhIFNbeta-1a mainly covalent, homogeneous (ca. 100 nm) aggregates. Reformulated rhIFNbeta-1a was essentially aggregate-free. All products induced BABs and NABs in wild-type mice. Immunogenicity in the transgenic mice was product dependent. RhIFNbeta-1b showed the highest and reformulated rhIFNbeta-1a the lowest immunogenicity. In contrast with wild-type mice, transgenic mice did not show NABs, nor did they respond to the rechallenge., Conclusions: The immunogenicity of the products in transgenic mice, unlike in wild-type mice, varied. In the transgenic mice, neither NABs nor immunological memory developed. The immunogenicity of rhIFNbeta in a model reflecting the human immune system depends on the presence and the characteristics of aggregates.

Published
2010
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43. Immunological mechanism underlying the immune response to recombinant human protein therapeutics.

Author

Sauerborn M, Brinks V, Jiskoot W, and Schellekens H

Subjects
Animals, Antibodies blood, B-Lymphocytes immunology, Erythropoietin immunology, Humans, Insulin immunology, Lymphocyte Activation, Thymus Gland physiology, Recombinant Proteins immunology, Recombinant Proteins therapeutic use
Abstract

Recombinant human (rhu) protein therapeutics are powerful tools to treat several severe diseases such as multiple sclerosis and diabetes mellitus, among others. A major drawback of these proteins is the production of anti-drug antibodies (ADAs). In some cases, these ADAs have neutralizing capacity and can interfere with the efficacy and safety of the drug. Little is known about the immunological mechanisms underlying the unwanted immune response against human homolog protein therapeutics. This article aims to provide current insights into recent immunological developments and to link this with regard to production of ADAs. A particular focus is given to aggregates being present in a rhu protein formulation and their impact on the immune system, subsequently leading to breakage of tolerance and formation of ADAs. Aggregation is one of the key factors in immunogenicity and by reducing aggregation one can reduce immunogenicity and make drugs safer and more efficient., (Copyright 2009 Elsevier Ltd. All rights reserved.)

Published
2010
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44. Hybrid transgenic immune tolerant mouse model for assessing the breaking of B cell tolerance by human interferon beta.

Author

van Beers MM, Sauerborn M, Gilli F, Hermeling S, Brinks V, Schellekens H, and Jiskoot W

Subjects
Animals, Antibodies, Neutralizing biosynthesis, B-Lymphocytes immunology, Chimera, Humans, Immune Tolerance, Interferon-beta administration & dosage, Mice, Mice, Inbred C57BL, Mice, Transgenic, Polyethylene Glycols metabolism, Protein Binding, Recombinant Proteins administration & dosage, Antibodies, Neutralizing blood, Enzyme-Linked Immunosorbent Assay, Interferon-beta immunology, Recombinant Proteins immunology
Abstract

To date, the therapeutic efficacy of recombinant human proteins is limited by their potential to break B cell tolerance in patients. The formation of neutralising antibodies (NABs) directed against recombinant human interferon beta (rhIFNbeta) is associated with a decrease in the therapeutic effect of the protein. For this reason, there is a need to study factors that can cause the immunogenicity of rhIFNbeta. Transgenic C57Bl/6 mice that are immune tolerant for human interferon beta (hIFNbeta) have been employed in a mouse model for assessing the breaking of immune tolerance by rhIFNbeta. In this study, we used the original C57Bl/6 mouse model as well as the hybrid offspring from crossings of transgenic C57Bl/6 mice with wildtype FVB/N mice to study the immunogenicity of three commercial rhIFNbeta products, Rebif, Avonex and Betaferon. As determined by ELISA, wildtype C57Bl/6 mice failed to form binding antibodies (BABs) against Rebif and Avonex formulated with human serum albumin. Because not all interferon beta products induce antibodies in wildtype C57Bl/6 mice, the transgenic C57Bl/6 mice cannot be used to study the breaking of tolerance by these products. However, the crossing of transgenic C57Bl/6 mice with FVB/N mice resulted in wildtype hybrid offspring in which all products were immunogenic and transgenic hybrid offspring that showed immune tolerance for hIFNbeta. Thus, these C57Bl/6 x FVB/N hybrid transgenic mice can be used to study the breaking of immune tolerance for all rhIFNbeta products. Of the three products, only Betaferon was able to break immune tolerance in the transgenic hybrids. With an MxA gene expression inhibition assay, NABs were detected in Betaferon treated wildtype hybrid mice, but not in transgenic hybrid mice, indicating a distinct immune mechanism in wildtype and transgenic mice. A pegylated rhIFNbeta-1a variant, PEG-rhIFNbeta-1a, induced antibodies in wildtype hybrid mice, but did not break the immune tolerance of transgenic hybrid mice. This suggests that pegylation did not affect the potential of rhIFNbeta-1a to break B cell tolerance., (Copyright 2009 Elsevier B.V. All rights reserved.)

Published
2010
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45. Non-invasive stress-free application of glucocorticoid ligands in mice.

Author

Dalm S, Brinks V, van der Mark MH, de Kloet ER, and Oitzl MS

Subjects
Adrenalectomy, Animals, Avena, Blood Glucose metabolism, Dose-Response Relationship, Drug, Glucocorticoids agonists, Glucocorticoids antagonists & inhibitors, Hormone Antagonists administration & dosage, Hormone Antagonists pharmacology, Hypothalamo-Hypophyseal System drug effects, Injections, Intraperitoneal, Ligands, Mice, Mice, Inbred C57BL, Mifepristone administration & dosage, Mifepristone pharmacology, Pharmaceutical Vehicles, Receptors, Glucocorticoid antagonists & inhibitors, Stress, Psychological physiopathology, Glucocorticoids pharmacology
Abstract

Most drug delivery procedures induce stress, which might interfere with the pharmacological action of the drug and behaviour. Stress is deduced from high and long-lasting elevations of the hormone corticosterone. We set out to develop a non-invasive, stress-free method of drug delivery in mice. Validation consisted of delivery of glucocorticoid ligands via oats to male C57BL/6J mice. Oat consumption induced a small increase in corticosterone concentrations after 15 min (<50 ng/ml) that returned to low resting levels at t=30 (<10 ng/ml). Gavage and intraperitoneal (i.p.) vehicle injections resulted in long-lasting corticosterone elevations (>100 ng/ml at t=30 and approximately 50 ng/ml at t=60 min after delivery). Adding corticosterone to oats resulted in threefold higher plasma corticosterone in the 15.0-mg/kg group (+/-250 ng/ml) compared to the 4.5-mg/kg group at t=30 and 90. Application of the glucocorticoid receptor antagonist RU38486 (200 mg/kg) elevated plasma corticosterone for at least 8h. Additional swimming increased corticosterone even further. Presumably, already the small oat-consumption-induced increase of corticosterone requires negative feedback via glucocorticoid receptors. In conclusion, the context-dependent and dose-controlled application of drugs via oats avoids confounding strong stress system activation and makes it suitable for studies on learning and memory processes.

Published
2008
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46. Strain specific fear behaviour and glucocorticoid response to aversive events: modelling PTSD in mice.

Author

Brinks V, de Kloet ER, and Oitzl MS

Subjects
Animals, Conditioning, Classical, Corticosterone blood, Fear physiology, Individuality, Male, Memory physiology, Mice, Mice, Inbred BALB C, Mice, Inbred C57BL, Species Specificity, Behavior, Animal physiology, Fear psychology, Glucocorticoids metabolism
Abstract

"Pavlovian" fear conditioning in rodents allows studying the formation and extinction of fear memories. Male C57BL/6J but not BALB/c mice showed differential fear memory performance expressed as freezing and scanning behaviour for context and cue. Glucocorticoid stress hormones modulate the processing of fear-related stimuli. The augmented corticosterone response of BALB/c mice to conditioning and testing, therefore, might have contributed to the strain-dependent formation of fear memories. We propose that modulation of extinction processes by glucocorticoids can be relevant in modelling anxiety disorders.

Published
2008
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47. Emotion and cognition in high and low stress sensitive mouse strains: a combined neuroendocrine and behavioral study in BALB/c and C57BL/6J mice.

Author

Brinks V, van der Mark M, de Kloet R, and Oitzl M

Abstract

Emotionally arousing experiences and stress influence cognitive processes and vice versa. Understanding the relations and interactions between these three systems forms the core of this study. We tested two inbred mouse strains (BALB/c, C57BL/6J; male; 3-month-old) for glucocorticoid stress system markers (expression of MR and GR mRNA and protein in hippocampus, amygdala, and prefrontal cortex; blood plasma corticosterone), used behavioral tasks for emotions and cognitive performance (elevated plus maze, holeboard) to assess the interdependence of these factors. We hypothesize that BALB/c mice have a stress-vulnerable neuroendocrine phenotype and that emotional expressions in BALB/c and C57BL/6J mice will differentially contribute to learning and memory. We applied factor analyses on emotional and cognitive parameters to determine the behavioral structure of BALB/c and C57BL/6J mice. Glucocorticoid stress system markers indeed show that BALB/c mice are more stress-vulnerable than C57BL/6J mice. Moreover, emotional and explorative factors differed between naïve BALB/c and C57BL/6J mice. BALB/c mice display high movement in anxiogenic zones and high risk assessment, while C57BL/6J mice show little movement in anxiogenic zones and display high vertical exploration. Furthermore, BALB/c mice are superior learners, showing learning related behavior which is highly structured and emotionally biased when exposed to a novel or changing situation. In contrast, C57BL/6J mice display a rather "chaotic" behavioral structure during learning in absence of an emotional factor. These results show that stress vulnerability coincides with more emotionality, which drives well orchestrated goal directed behavior to the benefit of cognition. Both phenotypes have their advantage depending on environmental demands.

Published
2007
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48. Differential MR/GR activation in mice results in emotional states beneficial or impairing for cognition.

Author

Brinks V, van der Mark MH, de Kloet ER, and Oitzl MS

Subjects
Adrenal Cortex Hormones administration & dosage, Adrenalectomy, Animals, Anxiety blood, Anxiety metabolism, Cognition Disorders blood, Corticosterone blood, Emotions drug effects, Male, Mice, Mice, Inbred C57BL, Receptors, Glucocorticoid agonists, Receptors, Mineralocorticoid agonists, Cognition physiology, Cognition Disorders metabolism, Emotions physiology, Receptors, Glucocorticoid metabolism, Receptors, Mineralocorticoid metabolism
Abstract

Corticosteroids regulate stress response and influence emotion, learning, and memory via two receptors in the brain, the high-affinity mineralocorticoid (MR) and low-affinity glucocorticoid receptor (GR). We test the hypothesis that MR- and GR-mediated effects interact in emotion and cognition when a novel situation is encountered that is relevant for a learning process. By adrenalectomy and additional constant corticosterone supplement we obtained four groups of male C57BL/6J mice with differential chronic MR and GR activations. Using a hole board task, we found that mice with continuous predominant MR and moderate GR activations were fast learners that displayed low anxiety and arousal together with high directed explorative behavior. Progressive corticosterone concentrations with predominant action via GR induced strong emotional arousal at the expense of cognitive performance. These findings underline the importance of a balanced MR/GR system for emotional and cognitive functioning that is critical for mental health.

Published
2007
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