Induction of Complement-Fixing Autoantibodies against Type VII Collagen Results in Subepidermal Blistering in Mice

Sitaru, Cassian; Chiriac, Mircea T.; Mihai, Sidonia; Büning, Jürgen; Gebert, Andreas; Ishiko, Akira; Zillikens, Detlef

doi:10.4049/jimmunol.177.5.3461

Cited by 141 publications

(203 citation statements)

References 61 publications

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“…We also used an Fcγ receptor-dependent skin-blistering disease caused by collagen type VII-specific autoantibodies (36) to evaluate the efficacy of s4-IVIg. Prophylactic dosing with IVIg between 0.1 and 1 g/kg at the onset of the disease (day 4) resulted in a clear dose-response within this dose range, which was measured by the percentage of affected body area (Fig.…”

Section: Optimization Of Sialylation Process: Minimizing Undesired Momentioning

confidence: 99%

Controlled tetra-Fc sialylation of IVIg results in a drug candidate with consistent enhanced anti-inflammatory activity

Washburn

Schwab

Ortiz

et al. 2015

Proc. Natl. Acad. Sci. U.S.A.

189

152

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Despite the beneficial therapeutic effects of intravenous immunoglobulin (IVIg) in inflammatory diseases, consistent therapeutic efficacy and potency remain major limitations for patients and physicians using IVIg. These limitations have stimulated a desire to generate therapeutic alternatives that could leverage the broad mechanisms of action of IVIg while improving therapeutic consistency and potency. The identification of the important anti-inflammatory role of fragment crystallizable domain (Fc) sialylation has presented an opportunity to develop more potent Ig therapies. However, translating this concept to potent anti-inflammatory therapeutics has been hampered by the difficulty of generating suitable sialylated products for clinical use. Therefore, we set out to develop the first, to our knowledge, robust and scalable process for generating a well-qualified sialylated IVIg drug candidate with maximum Fc sialylation devoid of unwanted alterations to the IVIg mixture. Here, we describe a controlled enzymatic, scalable process to produce a tetra-Fc-sialylated (s4-IVIg) IVIg drug candidate and its qualification across a wide panel of analytic assays, including physicochemical, pharmacokinetic, biodistribution, and in vivo animal models of inflammation. Our in vivo characterization of this drug candidate revealed consistent, enhanced anti-inflammatory activity up to 10-fold higher than IVIg across different animal models. To our knowledge, this candidate represents the first s4-IVIg suitable for clinical use; it is also a valuable therapeutic alternative with more consistent and potent anti-inflammatory activity.IVIg | sialylation | antibody | inflammation | autoimmune disease

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Section: Optimization Of Sialylation Process: Minimizing Undesired Momentioning

confidence: 99%

Controlled tetra-Fc sialylation of IVIg results in a drug candidate with consistent enhanced anti-inflammatory activity

Washburn

Schwab

Ortiz

et al. 2015

Proc. Natl. Acad. Sci. U.S.A.

189

152

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“…Sections were observed by fluorescence microscopy (Keyence, Osaka, Japan). Neutrophil infiltration in the skin was detected by immunohistochemistry (IHC) as described earlier with modifications (20). Sixmicrometer frozen skin sections were incubated with biotin-conjugated Ly-6G (1:200 dilution) Ab at 37˚C for 1 h. Subsequently, sections were incubated with Ultra-Sensitive ABC Peroxidase Staining Kit (Thermo Scientific Pierce Protein Research Products) at room temperature (RT) for 0.5 h and were developed by 3,39-diaminobenzidine (Merck, Darmstadt, Germany).…”

Section: If Microscopy Immunohistochemistry Immunoblot and Elisa Amentioning

confidence: 99%

“…Regarding the cellular requirements of autoantibody production, these models clearly documented a dependency on both B cells and CD4 T cells (15)(16)(17)(18). In principle, immunizationinduced models of AIBD (19)(20)(21) allow for investigating the cellular and molecular requirements that lead to loss of tolerance and subsequent autoantibody production. Yet, so far, detailed investigations on the cellular requirements in the early pathogenesis of these animal models had not been performed.…”

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confidence: 99%

B Cells, Dendritic Cells, and Macrophages Are Required To Induce an Autoreactive CD4 Helper T Cell Response in Experimental Epidermolysis Bullosa Acquisita

Iwata

Bieber

Tiburzy

et al. 2013

The Journal of Immunology

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In autoimmune bullous dermatoses (AIBD), autoantibodies induce blisters on skin or mucous membranes, or both. Mechanisms of continued autoantibody production and blistering have been well characterized using AIBD animal models. Mechanisms leading to the initial autoantibody production, however, have not been investigated in detail. Epidermolysis bullosa acquisita (EBA) is an AIBD associated with autoantibodies to type VII collagen (COL7). The majority of EBA patients’ sera recognize the noncollagenous domain 1, including the von Willebrand factor A–like domain 2 (vWFA2). In experimental EBA induced by immunization with GST-COL7, disease manifestation depended on the genetic background, a Th1 polarization, and the GST-tag. In this model, nude mice neither produced autoantibodies nor blisters. It has remained uncertain which APC and T cell subsets are required for EBA induction. We established a novel EBA model by immunization with vWFA2 fused to intein (lacking the GST-tag). All tested mouse strains developed autoantibodies, but blisters were exclusively observed in mice carrying H2s. In immunized mice, CD4 T cells specific for vWFA2 were detected, and their induction required presence of B cells, dendritic cells, and macrophages. Anti-vWFA2 autoantibodies located at the lamina densa bound to the dermal side of salt-split skin and induced blisters when transferred into healthy mice. Absence of CD8 T cells at time of immunization had no effect, whereas depletion of CD4 T cells during the same time period delayed autoantibody production and blisters. Collectively, we demonstrate the pathogenic relevance of Abs targeting the vWFA2 domain of COL7 and show the requirement of APC-induced CD4 T cells to induce experimental EBA.

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“…In addition, IgA antitype VII collagen reactivity, either exclusively or in combination with IgG autoantibodies, is observed in 50-60% of patients [26,27,66]. The pathogenic relevance of antibodies against type VII collagen has clearly been shown in several in vivo and in vitro models [67][68][69][70][71] reviewed in [6]. Incubation of cryosections of normal human skin with sera of EBA patients followed by incubation with neutrophils from healthy volunteers leads to dermal-epidermal split formation [69].…”

Section: Pathophysiologymentioning

confidence: 99%

“…the antitype VII collagen-mediated tissue destruction. To investigate the loss of tolerance to type VII collagen, mice were immunized with recombinant fragments of NC1 domain, which raised murine antitype VII collagen IgG that resulted in a long-lasting autoimmune skin disease resembling human EBA [68,74]. These animal models were subsequently used to show the pathogenic relevance of complement activation at the epidermal BMZ, neutrophils, CD18-mediated extravasation, FcγRIV, heat-shock protein 90, the glycosylation status of antitype VII collagen IgG, IL-1β, IL-6, GM-CSF, Erk 1/2, CXCL1/2, p38, Akt, RORa, HSP90, gene expression in myeloid cells, and the skin microbiome [75][76][77][78][79][80][81][82][83][84].…”

Section: Pathophysiologymentioning

confidence: 99%

Clinical features and diagnosis of epidermolysis bullosa acquisita

Vorobyev

Ludwig

Schmidt

2016

Expert Review of Clinical Immunology

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Introduction: Epidermolysis bullosa acquisita (EBA) is a rare autoimmune blistering disease of skin and mucous membranes. EBA is caused by autoantibodies against type VII collagen, which is a major component of anchoring fibrils, attaching epidermis to dermis. Binding of autoantibodies to type VII collagen leads to skin fragility and, finally, blister formation. The clinical picture of EBA is polymorphic, with several distinct phenotypes being described. Despite recent progress in understanding the pathophysiology of EBA, its diagnosis is still challenging. Areas covered: This review provides an update on the clinical manifestations and diagnostic methods of EBA. We searched PubMed using the terms 'epidermolysis bullosa acquisita' covering articles in English between 1 January 2005 and 31 May 2016. Relevant older publications were retrieved form cited literature. Expert commentary: While the clinical picture is highly variable, diagnosis relies on direct immunofluorescence (IF) microscopy of a perilesional skin biopsy. Linear deposits of IgG, IgA and/or C3 along the dermal-epidermal junction with an u-serrated pattern are diagnostic for EBA alike the detection of serum autoantibodies against type VII collagen. Several test systems for the serological diagnosis of EBA have recently become widely available. In some patients, sophisticated diagnostic approaches only available in specialized centers are required. ARTICLE HISTORY

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Induction of Complement-Fixing Autoantibodies against Type VII Collagen Results in Subepidermal Blistering in Mice

Cited by 141 publications

References 61 publications

Controlled tetra-Fc sialylation of IVIg results in a drug candidate with consistent enhanced anti-inflammatory activity

Controlled tetra-Fc sialylation of IVIg results in a drug candidate with consistent enhanced anti-inflammatory activity

B Cells, Dendritic Cells, and Macrophages Are Required To Induce an Autoreactive CD4 Helper T Cell Response in Experimental Epidermolysis Bullosa Acquisita

Clinical features and diagnosis of epidermolysis bullosa acquisita

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