Structural Characterization and Immunogenicity in Wild-Type and Immune Tolerant Mice of Degraded Recombinant Human Interferon Alpha2b

Hermeling, Suzanne; Aranha, Liliana; Damen, Johan; Slijper, Monique; Schellekens, Huub; Crommelin, Daan J.A.; Jiskoot, Wim

doi:10.1007/s11095-005-8177-9

Cited by 129 publications

(123 citation statements)

References 19 publications

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“…13 Low aggregate content is especially crucial in pharmaceutical formulations as aggregates here may elicit an inflammatory immune response to neutralize the aggregate. 14 This would not only diminish the effect of the drug itself but could also lead to more serious adverse effects related to cross-reactivity with autologous proteins. 15,16 In this study, we used the monoclonal IgG1 antibody Rituximab 17 as a model system to better understand the mechanisms leading to the formation of large aggregates when incubating a multidomain protein under weak thermal stress.…”

Section: Introductionmentioning

confidence: 99%

Aggregation of a multidomain protein: A coagulation mechanism governs aggregation of a model IgG1 antibody under weak thermal stress

et al. 2010

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Using an IgG1 antibody as a model system, we have studied the mechanisms by which multidomain proteins aggregate at physiological pH when incubated at temperatures just below their lowest thermal transition. In this temperature interval, only minor changes to the protein conformation are observed. Light scattering consistently showed two coupled phases: an initial fast phase followed by several hours of exponential growth of the scattered intensity. This is the exact opposite of the lagtime behavior typically observed in protein fibrillation. Dynamic light scattering showed the rapid formation of an aggregate species with a hydrodynamic radius of about 25 nm, which then increased in size throughout the experiment. Theoretical analysis of our light scattering data showed that the aggregate number density goes through a maximum in time providing compelling evidence for a coagulation mechanism in which aggregates fuse together. Both the analysis as well as size-exclusion chromatography of incubated samples showed the actual increase in aggregate mass to be linear and reach saturation long before all molecules had been converted to aggregates. The CH2 domain is the only domain partly unfolded in the temperature interval studied, suggesting a pivotal role of this least stable domain in the aggregation process. Our results show that for multidomain proteins at temperatures below their thermal denaturation, transient unfolding of a single domain can prime the molecule for aggregation, and that the formation of large aggregates is driven by coagulation.

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Section: Introductionmentioning

confidence: 99%

Aggregation of a multidomain protein: A coagulation mechanism governs aggregation of a model IgG1 antibody under weak thermal stress

et al. 2010

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“…15,16 Expression of human FVIII during this period should therefore lead to the depletion of high-avidity human FVIII-specific T cells and result in specific immune tolerance toward human FVIII. Similar genetically engineered mouse models were described for human insulin analogs, 17 modified human tissue plasminogen activator variants, 18 human IFNs, 19,20 human Fas ligand inhibitory protein (decoy receptor 3, DcR3), 21 and a mutant of human FVIII. 22 Transgenic mouse models for human IFN␣2b (hIFN␣2b) and human IFN␤ (hIFN␤) 19,20 were shown to be predictive of the human immune response, because commercially available hIFN␤ drugs that were found to induce antibodies in a large number of patients were shown to break immune tolerance in these mice.…”

Section: Introductionmentioning

confidence: 99%

“…Similar genetically engineered mouse models were described for human insulin analogs, 17 modified human tissue plasminogen activator variants, 18 human IFNs, 19,20 human Fas ligand inhibitory protein (decoy receptor 3, DcR3), 21 and a mutant of human FVIII. 22 Transgenic mouse models for human IFN␣2b (hIFN␣2b) and human IFN␤ (hIFN␤) 19,20 were shown to be predictive of the human immune response, because commercially available hIFN␤ drugs that were found to induce antibodies in a large number of patients were shown to break immune tolerance in these mice. 19 In the present study, we describe the selection and characterization of a transgenic mouse line that is immunologically tolerant to native human FVIII but is still able to mount an antibody response to human FVIII when challenged with a modified FVIII protein that possesses increased immunogenicity.…”

Section: Introductionmentioning

confidence: 99%

“…39 Therefore, the difference in the levels of human F8 cDNA and human F8 mRNA found after successful gene-therapy approaches and after transgenic expression of human F8 cDNA are likely to be substantial. There are several other examples of transgenic mouse models that are immunologically tolerant to specific human proteins such as insulin, 17 IFNs,19,20 or factor IX, 48 but lack detectable human protein in the circulation. Moreover, Connely et al 49 demonstrated that the lack of circulating FVIII protein observed after gene therapy using a vector containing a human F8 cDNA driven by an albumin promoter was not necessarily associated with a lack of the production of functional human FVIII protein.…”

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confidence: 99%

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

Helden

Unterthurner

Hermann

et al. 2011

Blood

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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. (Blood. 2011; 118(13):3698-3707) IntroductionHemophilia A is an X-linked bleeding disorder that is caused by reduced function or lack of clotting factor VIII (FVIII). 1 Replacement of the missing protein is the current standard of care for patients. However, the short half-life of FVIII, ϳ 7-17 hours, 2 makes frequent treatment necessary. Current efforts focus on the development of longer-acting FVIII concentrates, which should decrease the required treatment frequency and therefore improve the quality of life for patients. Recently described approaches in the development of longer-acting concentrates are based on strategies that have been successfully applied to other therapeutic proteins: chemical modifications such as the addition of polyethylene glycol (PEG) polymers, polysialic acids, or hydroxyethyl starch 3,4 ; alternative formulations with PEG-modified liposomes 3 ; and fusion to the Fc part of human IgG. 5 In addition, molecular modifications of the FVIII protein aimed at increasing the duration of its cofactor activity or reducing its clearance in vivo have been reported. 3 Any chemical or molecular modification of the FVIII protein can potentially increase its immunogenic potential. Modifications could generate neo-epitopes for both B and T cells or may induce altered structures that could bind and trigger receptors expressed on cells of the innate immune system, thereby amplifying potential anti-FVIII antibody responses. 6 Finally, modifications could generate repetitive epitopes for B cells that might cause the activation and differentiation of B cells and the subsequent production of antibodies without the requirement for T-cell help. 7,8 Therefore, the potential impact that any...

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“…Immunogenicity assays have shown that the nature of the aggregate and the type of protein are critical for eliciting an immune response as seen in several cases, IFN-␣ (9,(15)(16)(17), FVIII (18,19), and recombinant human growth hormone (20). Metal-catalyzed aggregates of IFN-␣ showed the highest level of response and were able to break the tolerance of transgenic mice (9,(15)(16)(17), whereas heat-aggregated FVIII was found to be less immunogenic than the monomeric protein (18,19).…”

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confidence: 99%

Classification and Characterization of Therapeutic Antibody Aggregates

Joubert

Luo

Nashed-Samuel

et al. 2011

Journal of Biological Chemistry

268

263

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A host of diverse stress techniques was applied to a monoclonal antibody (IgG 2 ) to yield protein particles with varying attributes and morphologies. Aggregated solutions were evaluated for percent aggregation, particle counts, size distribution, morphology, changes in secondary and tertiary structure, surface hydrophobicity, metal content, and reversibility. Chemical modifications were also identified in a separate report (Luo, Q., Joubert, M. K., Stevenson, R., Narhi, L. O., and Wypych, J. (2011) J. Biol. Chem. 286, 25134 -25144). Aggregates were categorized into seven discrete classes, based on the traits described. Several additional molecules (from the IgG 1 and IgG 2 subtypes as well as intravenous IgG) were stressed and found to be defined with the same classification system. The mechanism of protein aggregation and the type of aggregate formed depends on the nature of the stress applied. Different IgG molecules appear to aggregate by a similar mechanism under the same applied stress. Aggregates created by harsh mechanical stress showed the largest number of subvisible particles, and the class generated by thermal stress displayed the largest number of visible particles. Most classes showed a disruption of the higher order structure, with the degree of disorder depending on the stress process. Particles in all classes (except thermal stress) were at least partially reversible upon dilution in pH 5 buffer. High copper content was detected in isolated metal-catalyzed aggregates, a stress previously shown to produce immunogenic aggregates. In conclusion, protein aggregates can be a very heterogeneous population, whose qualities are the result of the type of stress that was experienced.

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Structural Characterization and Immunogenicity in Wild-Type and Immune Tolerant Mice of Degraded Recombinant Human Interferon Alpha2b

Cited by 129 publications

References 19 publications

Aggregation of a multidomain protein: A coagulation mechanism governs aggregation of a model IgG1 antibody under weak thermal stress

Aggregation of a multidomain protein: A coagulation mechanism governs aggregation of a model IgG1 antibody under weak thermal stress

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

Classification and Characterization of Therapeutic Antibody Aggregates

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