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From the Cover
BIOLOGICAL SCIENCES / MEDICAL SCIENCES
IgG glycan hydrolysis by a bacterial enzyme as a therapy against autoimmune conditions

Mattias Collin^*, Oonagh Shannon, and Lars Björck

Division of Infection Medicine, Department of Clinical Sciences, Lund University, SE-22184 Lund, Sweden

Edited by Emil C. Gotschlich, The Rockefeller University, New York, NY, and approved January 22, 2008 (received for review November 29, 2007)

	Abstract

Top Abstract Results Discussion Materials and Methods Acknowledgments. References

 
EndoS from Streptococcus pyogenes efficiently hydrolyzes the functionally important and conserved N-linked glycan of IgG in human blood. Repeated i.v. administration of EndoS in rabbits completely hydrolyzes the glycans of the whole IgG pool, despite the generation of anti-EndoS antibodies. EndoS administration had no apparent effects on the health of the animals. EndoS hydrolysis of the IgG glycan has profound effects on IgG effector functions, such as complement activation and Fc receptor binding, suggesting that the enzyme could be used as an immunomodulatory therapeutic agent against IgG-mediated diseases. We demonstrate here that EndoS indeed has a protective effect in a mouse model of lethal IgG-driven immune (or idiopathic) thrombocytopenic purpura. EndoS pretreatment of pathogenic antibodies inhibits the development of disease, and the enzyme also rescues mice from already established disease when severe thrombocytopenia and s.c. bleeding have developed. These results identify EndoS as a potential therapeutic agent against diseases where pathogenic IgG antibodies are important and further emphasize antibody glycans as possible targets in future therapies against antibody-mediated autoimmune conditions.

autoimmunity | immunomodulation | Streptococcus pyogenes | endoglycosidase | glycosylation

View larger version (41K): [in this window] [in a new window]   Fig. 1. Structure and glycosylation of IgG. (A) Schematic representation of the fully substituted IgG heavy-chain glycan. S2 indicates the fully sialylated glycoform G0, and brackets indicate the extent of the G0 glycoform. LCA indicates the binding site for the LCA used in lectin experiments and EndoS the cleavage site for the enzyme. (B) Structural model of human IgG. IgG heavy chains are colored blue, and the light chains are colored red. Brackets indicate the antigen-binding Fab' portion and the Fc effector portion of IgG. Arrow indicates the two conserved glycans (yellow) attached to Asn-297 of the heavy chains. The model was generated by using VMD 1.8.5 from a model deposited in the Protein Data Bank by M. Clark (Cambridge University, Cambridge, U.K.).

Autoimmune disorders constitute a large group of diseases with various manifestations from mild to severe, but they all have in common that the immune system attacks and damages endogenous tissues and organs. Many autoimmune disorders have been thought to be largely dependent on the cellular branch of adaptive immunity mediated through T lymphocytes, but accumulating evidence suggests that B lymphocytes and autoantibodies are more important than previously appreciated for the development of disease (17). This also is true for acute and chronic organ-allograft rejection, where recent studies have shown that alloantibodies fixating complement on the allograft account for a substantial portion of graft-rejection episodes (18). Therapies, especially for the severe cases of both autoantibody-mediated autoimmune diseases and acute allograft rejection, focus on reducing antibody titers and production through plasmapheresis, immunosuppressants, antibodies directed toward B cells, and IVIG.

Immune (or idiopathic) thrombocytopenic purpura (ITP) is a relatively common autoimmune disorder, with an incidence of 5.5–6.6 per 100,000 people (19). ITP is caused by autoantibodies directed toward antigens on platelets (20), and platelets coated with IgG autoantibodies are cleared by FcR expressing tissue macrophages predominantly in the liver and spleen, causing the characteristic low platelet count and mucocutaneous bleeding (21). Current treatment of ITP focuses on reducing the production of pathogenic IgG and on reduction of platelet clearance by IVIG, splenectomy, corticosteroids, nonspecific immunosuppressants, monoclonal antibodies against B and T cells, and plasmapheresis (21, 22).

Because of the EndoS-specificity for IgG, its effects on IgG effector functions, and the importance of IgG in autoimmune disorders and allograft rejection, we hypothesized that EndoS could be used in vivo as a potential therapeutic agent against antibody-mediated diseases. This hypothesis was further stimulated by our recent finding that pretreatment of arthritogenic autoantibodies with EndoS abrogates the development of disease in a mouse model of collagen-induced arthritis (23). The IgG-specific protease IdeS also has been shown to be efficient in a similar model system (24) and in the mouse model of ITP used in this study (25). For EndoS to work as a useful agent against pathological IgG in vivo, it needs to fulfill several criteria. For instance, it cannot have any major adverse effects on animals; it must be active in a complex environment, such as human blood or the circulation of a live animal at reasonable concentrations; and, finally, it should work as a treatment in an animal model of an antibody-mediated disease.

Here we show that purified EndoS at low concentrations efficiently hydrolyzes the glycan on IgG in human blood, that EndoS can be injected i.v. in rabbits without adverse effects, and that EndoS at low concentrations hydrolyzes the glycans of the entire IgG pool in rabbits despite repeated administration and generation of antibodies toward EndoS. Furthermore, in a mouse model of lethal IgG-mediated thrombocytopenia, EndoS treatment inhibits the development of disease, but also rescues mice from already established disease with severe thrombocytopenia and s.c. bleeding. These results identify EndoS as a potential therapeutic agent in diseases where IgG antibodies play an important pathogenic role.

	Results

Top Abstract Results Discussion Materials and Methods Acknowledgments. References

 
EndoS Efficiently Hydrolyzes the IgG Glycans in Human Blood. To function as a therapeutic agent against pathological IgG, EndoS needs to be active at low concentrations in whole human blood. To investigate this enzymatic activity, increasing final concentrations (0, 0.31, 0.63, 1.25, 2.5, 5, 10, and 20 µg/ml) of EndoS were incubated in heparinized human blood from healthy volunteers, followed by purification of IgG on immobilized protein G. There was no difference in binding efficiency to protein G between fully glycosylated IgG and EndoS-treated IgG (data not shown), which is in concordance with our previous findings for the IgG-binding protein H from S. pyogenes and protein A from Staphylococcus aureus (2). SDS/PAGE analysis of the samples showed that increasing concentrations of EndoS gradually shift the IgG heavy chain to an 3-kDa smaller apparent molecular mass and that almost no full-size heavy chain could be seen above a concentration of 2.5–5 µg/ml EndoS (Fig. 2A). The Lens culinaris agglutinin (LCA) lectin blot analysis of the same samples showed that increasing concentration of EndoS gradually gives a lower carbohydrate signal and that there is virtually no signal above EndoS concentrations of 2.5–5 µg/ml (Fig. 2B). We have previously shown that the lack of lectin signals corresponds well with complete IgG glycan hydrolysis as analyzed by mass spectroscopy (3). Furthermore, peak density analysis shows a dose–response curve, which flattens out to background levels around an EndoS concentration of 5 µg/ml (Fig. 2C). These results demonstrate that 5 µg/ml EndoS within 1 h completely hydrolyzes the IgG pool in human blood. Thus, EndoS shows a remarkably efficient hydrolysis of the functionally important IgG glycan in the complex environment of human blood.

View larger version (21K): [in this window] [in a new window]   Fig. 2. EndoS hydrolyzes IgG in whole human blood. (A) SDS/PAGE analysis of purified IgG from human blood incubated with increasing concentrations of EndoS. (B) LCA lectin blot analysis of purified IgG from whole human blood incubated with increasing concentrations of EndoS. (C) Densitometric analysis of the lectin blot on IgG purified from human blood incubated with increasing concentrations of EndoS. Values are presented as the percentage of signal from control sample incubated with buffer alone. Means and standard errors were calculated from three independent experiments using blood from three different donors.

View larger version (38K): [in this window] [in a new window]   Fig. 3. EndoS hydrolyzes IgG in vivo in rabbits. (A) SDS/PAGE (stain) and lectin blot analysis (LCA blot) of purified IgG from serum samples withdrawn from a representative rabbit at indicated time points after the first i.v. injection of 500 µg of EndoS (0 days). (B) SDS/PAGE (stain) and lectin blot analysis (LCA blot) of purified IgG from serum samples withdrawn from the rabbit at indicated time points after a second administration (35 days) of EndoS. (C) SDS/PAGE (stain) and lectin blot analysis (LCA blot) of purified IgG from serum samples withdrawn from the rabbit at indicated time points after a third administration (135 days) of EndoS. (D) Lectin blot analysis of total serum taken before (0) and 12 h (12) after the first injection of EndoS. ConA, Concavalin A; SNA, Sambucus nigra lectin. Arrow to the right indicates the position of the -chain of IgG.

None of the three rabbits showed any signs of disease after any of the EndoS injections as judged by normal weight gain and normal group behavior. Furthermore, the levels of protein G-purified total serum IgG were not significantly altered during the course of the experiment (data not shown). Taken together, these results show that low concentrations of EndoS efficiently hydrolyze the heavy-chain glycan on the whole-rabbit IgG pool in vivo without altering the IgG concentration or having any detectable activity on other serum glycoproteins. Furthermore, previous i.v. exposure to EndoS does not significantly affect the in vivo enzymatic activity of EndoS.

Because EndoS had full activity when injected repeatedly into rabbits, we wanted to determine the immune response against the enzyme. This immune response is of particular interest because most humans have been infected with S. pyogenes and carry antibodies against EndoS (27). Serum samples from rabbits were analyzed for reactivity against purified EndoS. Already before the first injection, there were antibodies reacting with EndoS in Western blot (Fig. 4Inset, day 0), suggesting that rabbits also are exposed to EndoS or a related molecule, giving rise to anti-EndoS IgG antibodies. There was only a slight increase in reactivity toward EndoS 10 days after injection (Fig. 4 Inset). Western blots were not practical to use for an analysis of samples obtained after the second and third injections because of very high signal levels (data not shown). Therefore, samples before and after all three injections also were analyzed by ELISA. This revealed that, just before the second injection of EndoS, the reactivity against EndoS was comparable or slightly higher than before the first injection, and the reactivity did not increase until 5 days after injection as determined by ELISA (Fig. 4, first and second injections). From days 5–10 after the second injection, the reactivity against EndoS gradually increased (Fig. 4, second injection, days 5–10). Before the third injection of EndoS, the reactivity against EndoS was slightly higher than before the second injection, and the reactivity did not increase during the first day after injection (Fig. 4, third injection, days 0–1). From days 5–10 after the third injection, the reactivity against EndoS increased dramatically (Fig. 4, third injection, days 5–10). These results indicate that there are antibodies directed toward EndoS in unexposed animals and that EndoS elicits an immune response in rabbits upon repeated i.v. exposure. However, these antibodies do not interfere with the activity of EndoS in the circulation during three consecutive administrations. Furthermore, repeated administration does not affect the 12-h circulation time (defined as the ability to detect EndoS) of the enzyme as analyzed by immunoprecipitation and Western blot analysis of EndoS from rabbit serum samples (data not shown).

View larger version (25K): [in this window] [in a new window]   Fig. 4. Rabbit antibody response to EndoS. Serum samples were withdrawn from the rabbit at indicated time points after the first (0 days), second (35 days), and third (135 days) injections of EndoS. Serum samples after the first (0 days), second (35 days), and third (135 days) injections were used as primary antisera in an ELISA experiment with immobilized EndoS. Increase in concentration (ng/ml) of anti-EndoS IgG compared with concentration before first injection is presented. One representative experiment is shown. (Inset) The serum samples after the first injection were used as primary antisera in a Western blot on separate membrane strips with SDS/PAGE-separated purified EndoS.

In a pilot experiment, three female BALB/c mice were injected with 1.2 mg of PLT-IgG, and platelet counts were followed over time by using flow cytometry and microscopy. This revealed that all three mice rapidly developed thrombocytopenia, and death occurred within 24 h after PLT-Ig administration (Fig. 5A).

View larger version (8K): [in this window] [in a new window]   Fig. 5. EndoS pretreatment of pathogenic IgG antibodies inhibits antibody-mediated thrombocytopenia in mice. (A) Female BALB/c mice (n = 3) received i.p. injections of rabbit anti-mouse platelet IgG (PLT-IgG). Blood samples were taken at regular intervals, and platelet counts were determined by using flow cytometry. (B) Survival plots of BALB/c mice injected with PLT-IgG that were pretreated with GST-EndoS (n = 4) or GST (n = 4). (C) Platelet counts over time as determined by flow cytometry on blood samples from mice that had received PLT-IgG pretreated with GST-EndoS.

View larger version (25K): [in this window] [in a new window]   Fig. 6. EndoS rescues mice from lethal IgG-mediated thrombocytopenia. (A) Survival plots of BALB/c mice injected with PLT-IgG, followed by GST-EndoS (n = 8) or GST (n = 8) treatment 3 h after PLT-IgG administration. (B) SDS/PAGE analysis (stain) and LCA lectin blot analysis (LCA blot) of IgG purified from GST-EndoS or GST-treated mice 24, 48, or 72 (only GST-EndoS) h after injection of PLT-Ig. (C) Blood samples were taken at regular intervals, and platelet counts were determined by using flow cytometry in mice that received GST-EndoS treatment. (D) Survival plots of BALB/c mice injected with PLT-Ig, followed by GST-EndoS (n = 7) or GST (n = 7) treatment at the onset of clear signs of intraabdominal bleeding (5–7 h after PLT-Ig administration).

	Discussion

Top Abstract Results Discussion Materials and Methods Acknowledgments. References

 
We have demonstrated that purified EndoS from S. pyogenes at low concentrations efficiently hydrolyzes the conserved N-linked glycan on IgG heavy chains in whole human blood. Assuming an IgG plasma concentration of 10 mg/ml, EndoS completely hydrolyzes the glycans of the IgG pool in 1 h at an EndoS:IgG ratio of 1:2,000. Of particular interest is the finding that EndoS has no detectable effects on other plasma proteins, and we have been able to show previously that, despite its activity on IgG, EndoS has no activity on the closely related molecules, IgA and IgM (2). The specificity of EndoS for the N-linked glycans of a specific glycoprotein (IgG) makes it stand out from the other known enzymes in family 18 of glycosyl hydrolases. Most of these enzymes, including EndoF_1–3 from Elizabethkingia meningoseptica (formerly Flavobacterium meningosepticum), are specific for certain glycan structures that can be attached to any protein or peptide and are enhanced by or require denaturation of the protein backbone (30). This is in complete contrast to EndoS, which exclusively hydrolyzes native IgG or IgG Fc, suggesting that the substrate specificity depends on protein–protein interactions between the enzyme and IgG Fc (2, 4). Furthermore, we have recently shown that EndoS does not interact with IgG lacking most of its heavy-chain glycans, suggesting a complex interaction between enzyme and substrate involving both protein–protein and protein–glycan interactions (6, 26).

Our in vivo experiments in rabbits show that EndoS efficiently hydrolyzes the heavy-chain glycans on the whole IgG pool without any noticeable adverse effects or signs of disease, and the glycan hydrolysis does not significantly alter the total plasma concentration of IgG. The glycosylation state has been shown to influence the proteolytic resistance of IgG (31). Therefore, our results suggest that the core N-acetylglucosamine (with or without a core fucose) provides comparable proteolytic resistance as intact IgG. Furthermore, the largely unchanged total IgG concentration might indicate that the interaction of IgG hydrolyzed by EndoS with the protective FcRn (32) is not altered in the same way as for the other FcRs (6).

Because EndoS hydrolysis of IgG does not affect the antigen-binding Fab portion, IgG functions such as neutralization of enzymes, and toxins are probably not affected. Furthermore, repeated administration and the development of anti-EndoS antibodies does not significantly reduce the circulation time and has only minor effects on the activity of the enzyme. A possible explanation for this is that other EndoS molecules rapidly hydrolyze antibodies directed toward EndoS, and EndoS–antigen complexes can therefore not be efficiently removed by the reticuloendothelial system. However, it should be noted that after the third injection, where there were high antibody titers against EndoS, IgG reactivity with lectin reappeared earlier than after the two prior injections. This finding is most likely due to a partial antibody-mediated removal of EndoS.

In the mouse model of ITP, EndoS had dramatic positive effects on the platelet count and survival, both when pathogenic antibodies were pretreated with the enzyme and when EndoS was administered early or late during the course of disease. In this model, in vivo hydrolysis of IgG glycans has been used as an experimental treatment of an autoimmune disease. The mechanisms underlying the positive effects of EndoS are, from a theoretical viewpoint, quite clear because we have previously shown that EndoS hydrolysis of IgG inhibits IgG of all subclasses from binding to FcRs and also reduces complement activation (5, 6). Not only does EndoS inhibit IgG from binding FcRs, but it also can release already FcR-bound IgG by hydrolysis of the heavy-chain glycan. It also should be noted that there seems to be one IgG–FcR interaction that is not affected like the others: EndoS-hydrolyzed IgG does, under certain circumstances, bind better to human FcRIIb than nonhydrolyzed IgG (6). In the context of antiinflammatory activity, this finding might be of relevance because IgG interactions with FcRIIb have been shown to be important for the antiinflammatory activity of IVIG that is used to treat autoimmune conditions (33, 34). Therefore, one could speculate that EndoS under certain circumstances may have a dual antiinflammatory activity by directly inhibiting the binding of pathogenic IgG to activating FcRs and shifting toward the inhibitory action mediated through FcRIIb.

The properties of EndoS make it an attractive alternative to current therapies of conditions involving pathogenic antibodies, especially in the light of several recent studies establishing the IgG glycan as a key to IgG effector modulation. This includes our own findings that EndoS hydrolysis of this glycan nearly abolishes complement activation through the classical pathway and reduces binding to FcRs on leukocytes (5, 6). Based on our current and previous observations, we suggest that EndoS could be used to treat conditions where IgG antibodies play a pathogenic role, including autoimmune diseases as exemplified here by ITP and acute antibody-mediated organ allograft rejections.

	Materials and Methods

Top Abstract Results Discussion Materials and Methods Acknowledgments. References

 
EndoS Activity in Human Blood. Recombinant untagged and GST-tagged EndoS were expressed and purified to 95% homogeneity as described (4). Untagged recombinant enzyme is designated EndoS throughout the article and the tagged form GST-EndoS. Increasing final concentrations (0, 0.31, 0.63, 1.25, 2.5, 5, 10, and 20 µg/ml) of EndoS was incubated in 500 µl of heparinized human blood from three different healthy volunteers with rotation end over end for 1 h at 37°C. Samples were centrifuged at 720 x g for 10 min at 4°C, followed by purification of total IgG in plasma by using protein G Sepharose according to the manufacturer's instructions (GE Healthcare Biosciences). Purified IgG was separated on SDS/10% PAGE, stained with Coomassie blue, or electroblotted onto PVDF (Immobilon-P; Millipore). Glycosylated IgG was detected by using 5 µg/ml biotinylated LCA lectin and 1 µg/ml streptavidin-horseradish peroxidase (Vector Laboratories) and SuperSignal West Pico peroxidase substrate (Pierce). Membranes were analyzed by using a Chemidoc XRS imaging system and Quantity One image analysis software (BioRad).

EndoS Activity in Rabbits. Swedish lop rabbits with a body weight of 3 kg were injected i.v. at days 0, 35, and 130 with 1 mg of EndoS, corresponding to an approximate EndoS:IgG ratio of 1:2,000 given that EndoS distributes in blood only. Animals were housed in an animal facility and were checked for signs of disease hourly for the first 12 h and daily for the duration of the study. After EndoS injections, serum samples were withdrawn at 0, 1, 2, 4, 6, 8, and 12 h, and 1, 2, 3, 4, 5, 6, 8, and 10 days. After injections 2 and 3, samples also were taken after 14 days. Serum IgG was analyzed for glycosylation status by using SDS/PAGE and lectin blot analysis as described above for human blood. Total serum protein glycosylation at 0 and 12 h after the first EndoS injection was analyzed by separation of 0.1 µl of serum on SDS/10% PAGE, blotting to PVDF, and detection by using 1 µg/ml biotinylated ConA or SNA (both from Vector Laboratories), 1 µg/ml streptavidin-horseradish peroxidase, and substrate as above. The Laboratory Animal Ethics Committee of Malmö/Lund has approved the animal experiments.

Detection of EndoS Antibodies in Rabbits. Purified untagged EndoS was separated on SDS/10% PAGE and electroblotted onto PVDF that was cut into 1.5-mm strips. Strips were incubated with 1:500 dilutions of serum samples from the first injection, followed by incubation with peroxidase-labeled goat anti-rabbit antibodies (Pierce). Strips were developed by using chemiluminescence as described above for lectin blots. For ELISA experiments, 2 µg of EndoS was used to coat microtiter plates (Nunc), followed by blocking with 20 mg/ml BSA in PBS. Sera from animals before EndoS injections and 0.5, 1, 5, and 10 days after injections were used as primary antiserum in serial dilutions of 1:100 to 1:200,000. Peroxidase-labeled goat anti-rabbit antibodies (Pierce) were used as secondary antibodies and ABTS (Roche) as a peroxidase substrate. A standard curve for rabbit IgG was generated by coating microtiter plates as above with serial dilutions of polyclonal rabbit IgG (Sigma–Aldrich) and peroxidase-labeled goat anti-rabbit antibodies as secondary antibodies. Plates were analyzed at 405 nm in a Victor3 multilabel reader (PerkinElmer).

Mouse Model of IgG-Mediated Thrombocytopenia. Rabbit antiserum against mouse platelets was purchased from Inter-Cell Technologies. The IgG fraction was isolated from this serum by using protein G Sepharose. Protein purity was confirmed by SDS/PAGE analysis, and protein concentration was determined by using advanced protein assay reagent (Cytoskeleton). For experiments using pretreated IgG, purified rabbit anti-mouse platelet IgG was incubated with GST-EndoS or GST, purified as described (4), at an enzyme to substrate ratio of 1:500 at 37°C for 24 h, followed by removal of GST-EndoS and GST on a glutathione-Sepharose (GE Healthcare). IgG glycan hydrolysis was confirmed by SDS/PAGE and lectin blotting using LCA as described above. Female BALB/c mice (20 g in body weight) were housed under standard conditions of light and temperature and were fed standard laboratory chow and water ad libitum. Then 1.2 mg of anti-mouse platelet IgG (untreated, EndoS-treated, or GST-treated) in 0.25 ml of PBS was administered to the animals by i.p. injection. Animals were monitored for mucocutaneous bleeds, physical activity, and isolation from the group, and the survival time was recorded.

Blood Sampling from Mice and Platelet Analysis. Immediately before the injection of rabbit anti-mouse platelet IgG and at regular intervals during the course of the experiment, blood samples were collected from mice. From the prewarmed tail vein, 5 µl of whole blood was collected into tubes containing 45 µl of 0.1 M sodium citrate/citric acid in PBS (pH 6.5). The platelet population in these blood samples was identified by flow cytometry. Samples were labeled with hamster anti-mouse CD-61 PE (BD Biosciences) for 10 min at room temperature; then 10 µl of SPHERO Rainbow Calibration Particles (BD Biosciences) were added to each tube to enable counting. The RBC populations were lysed by using Utilyse (Dako), and the samples were analyzed on a FacsCalibur flow cytometer (BD Biosciences) in the logarithmic mode. The platelet number in the blood samples after lysis of RBCs was confirmed by manual counting in a Neubauer chamber.

	Acknowledgments.

Top Abstract Results Discussion Materials and Methods Acknowledgments. References

 
We thank Ulla Johannesson for excellent technical assistance. This work was supported by Swedish Research Council Grants 2005-4791 (to M.C.) and 2005-7480 (to L.B.), the Swedish Government Funds for Clinical Research (L.B.), the Kock Foundation (M.C. and L.B.), the Jeansson Foundation (M.C.), the Zoégas Foundation (M.C.), the Bergvall Foundation (M.C.), the Österlund Foundation (M.C., O.S., and L.B.), the Groschinsky Foundation (M.C.), the Crafoord Foundation (M.C.), the Royal Physiografic Society (M.C and O.S.), the Hansa Medical AB (to L.B.), and a Swedish Research Council Assistant Professorship (to M.C.).

	Footnotes

 
*To whom correspondence should be addressed. E-mail: mattias.collin{at}med.lu.se

Freely available online through the PNAS open access option.

Author contributions: M.C., O.S., and L.B. designed research; M.C. and O.S. performed research; O.S. contributed new reagents/analytic tools; M.C., O.S., and L.B. analyzed data; and M.C. wrote the paper.

Conflict of interest statement: Hansa Medical, which funded this study in part, has filed a patent application on the in vivo use of EndoS. M.C., O.S., and L.B. are listed as inventors, and the application is pending.

This article is a PNAS Direct Submission.

See Commentary on page 4081.

© 2008 by The National Academy of Sciences of the USA

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