Therapeutic potential of deglycosylated antibodies.

Autoimmune destruction of self tissue is the consequential result of a convergence of several factors, both genetic and environmental, that effectively dislocates the immune system’s ability to tolerate selfantigens but simultaneously retains its focus on those perceived as foreign. Although many of these autoimmune targeted selfantigens are known, immune system triggers can be more elusive. Nevertheless, once autoimmunity has been initiated, what is clear is the role that immune complexes (IC) play as a significant driving force in maintaining chronic inflammation and subsequently pathology in many of these conditions. ICs are antibody/antigen assemblies, usually IgG antibody subtype, sometimes found systemically but primarily at the site of autoimmune selfantigen recognition. Nandakumar et al. have revealed a unique approach to the disruption of these pathogenic complexes (1). Nandakumar et al. used the mouse anticollagen type II (anti-CII) mediated-arthritis model to show that deglycosylated IgG, regardless of Fab antigen specificity, reduces inflammation in a dose-dependent manner (1). This finding suggests that deglycosylated IgG has a dominant suppressive effect on inflammation and points to a unique class of therapeutic immunoglobulins for the treatment of autoimmunity. Antibody deglycosylation was achieved by in vitro digestion with EndoS (endo-β-Nacetylglucosaminidase). EndoS is an immune evasion factor from Streptococcus pyogenes, which functions by cleaving the glycans from the fragment crystallizable (Fc) domain of IgG molecules (2, 3). EndoS is highly unusual in its lack of cross-reactivity to other glycoproteins and has a tight specificity for the biantennary glycans found on serum IgG (4). Hydrolysis of the Fc glycans by EndoS significantly reduces the binding to cellular receptors of the immune system to IgG (5). These Fc γ-receptors (FcγR) bind asymmetrically across the lower hinge region and the tips of the Cγ2 domains (6). Crystallographic analysis of the endoglycosidasetreated human IgG Fc shows a closed configuration incompatible with receptor binding (7); solution-phase biophysical analysis shows an increased radius of gyration (8). Taken together these studies demonstrate that the quaternary architecture of the Fc is perturbed upon deglycosylation (Fig. 1). Administration of EndoS has emerged as a promising route to the deactivation of autoimmune antibodies and the alleviation of autoimmunity (9–13). However, a recent study by Tradtrantip et al. has suggested that the administration of pathogenic antibodies directed to autoimmune epitopes that have undergone prior deglycosylation ex vivo can also inhibit antibody-dependent cellular cytotoxicity (14). Similar observations have been made in a murine model of fetal/neonatal alloimmune thrombocytopenia. Bakchoul et al. demonstrated that administration of maternal alloantibodies that have been deglycosylated ex vivo prevent destruction of fetal platelets by endogenous glycosylated autoantibodies (15). Nandakumar et al. have made a surprising and significant step by establishing that the deglycosylated antibody does not need to be epitope-specific (1). However, epitope-independent anti-inflammatory activity of deglycosylated IgG, although highly unusual, is upon first inspection somewhat contradictory with the observation of the loss of anti-inflammatory activity of intravenous Ig upon deglycosylation in themouse serum-transfer arthritis model (16). Intravenous Ig consists of pooled human serum IgG and is used as a broad antiinflammatory. However, different animal strains and the mechanism used for disease induction will both have an impact onwhich component of immune dysfunction is being tested. The anti-CII mediated-arthritis model adopted by Nandakumar et al. (1) allows for accurate timing of the administration of deglycosylated antibody at the point where IC formation is known to be occurring. It would be interesting to see if these effects could be reproduced within a CII model where endogenous autoantibodies are produced, and which might more closely resemble the challenges faced in the clinic. The anti-inflammatory mechanism of deglycosylated antibodies is of considerable interest. Although in the epitopedirected study by Tradtrantip et al. (14) the effect on antibody-dependent cellmediated cytotoxicity might be ascribed to a competition with deactivated Fc, the epitope-independent effect on IC formation Fig. 1. Deglycosylation of IgG Fc by EndoS. Crystal structure of human IgG1 Fc containing (A) native complextype glycans (19) and (B) the residual glycan following hydrolysis of the glycan by an endoglycosidase (6). The protein is depicted in gray cartoon with transparent surface; the carbohydrate moiety is depicted as orange spheres. The gray lines indicate the increased flexibility of the deglycosylated Fc (4).