Clustered O-Glycans of IgA1

Takahashi, Kazuo; Wall, Stephanie; Suzuki, Hitoshi; Smith, Anita; Hall, Stacy; Poulsen, Knud; Kilian, Mogens; Mobley, James A.; Julian, Bruce A.; Městecký, Jiří; Novák, Jan; Renfrow, Matthew B.

doi:10.1074/mcp.m110.001834

Cited by 91 publications

(79 citation statements)

References 53 publications

(96 reference statements)

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“…Galactose-deficient polymeric IgA 1 (Ale) was isolated from the plasma of a patient with multiple myeloma using salt precipitation, jacalin precipitation, IgG-depletion on an anti-IgG column and size-exclusion chromatography (37, 38). Heterogeneity of O -glycans of this IgA 1 was fully characterized by high-resolution mass spectrometry (39, 40). …”

Section: Methodsmentioning

confidence: 99%

The Combined Role of Galactose-Deficient IgA1 and Streptococcal IgA–Binding M Protein in Inducing IL-6 and C3 Secretion from Human Mesangial Cells: Implications for IgA Nephropathy

Schmitt

Ståhl

Olin

et al. 2014

The Journal of Immunology

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IgA nephropathy is characterized by mesangial cell proliferation and extracellular matrix expansion associated with immune deposits consisting of galactose-deficient polymeric IgA1 and C3. We have previously shown that IgA-binding regions of streptococcal M proteins co-localize with IgA in mesangial immune deposits in patients with IgA nephropathy. In the current study, the IgA-binding M4 protein from group A streptococcus was found to bind to galactose-deficient polymeric IgA1 with higher affinity than to other forms of IgA1, as shown by surface plasmon resonance and solid-phase immunoassay. The M4 protein was demonstrated to bind to mesangial cells not via the IgA-binding region but rather via the C-terminal region, as demonstrated by flow cytometry. IgA1 enhanced binding of M4 to mesangial cells, but not vice versa. Co-stimulation of human mesangial cells with M4 and galactose-deficient polymeric IgA1 resulted in a significant increase in IL-6 secretion compared to each stimulant alone. Galactose-deficient polymeric IgA1 alone, but not M4, induced C3 secretion from the cells and co-stimulation enhanced this effect. In addition, co-stimulation enhanced mesangial cell proliferation compared to each stimulant alone. These results indicate that IgA-binding M4 protein binds preferentially to galactose-deficient polymeric IgA1 and that these proteins together induce excessive pro-inflammatory responses and proliferation of human mesangial cells. Thus, tissue deposition of streptococcal IgA-binding M proteins may contribute to the pathogenesis of IgA nephropathy.

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Section: Methodsmentioning

confidence: 99%

The Combined Role of Galactose-Deficient IgA1 and Streptococcal IgA–Binding M Protein in Inducing IL-6 and C3 Secretion from Human Mesangial Cells: Implications for IgA Nephropathy

Schmitt

Ståhl

Olin

et al. 2014

The Journal of Immunology

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“…Furthermore, O-glycans still prove to be difficult to remove from the protein by both enzymatic and chemical procedures. 11–13 The most common methodology for characterizing proteins with multiple glycosylation sites is therefore by liquid chromatography–tandem mass spectrometry (LC-MS/MS) of protease-generated glycopeptides. Glycosylated species are then identified from masses that correspond to prior known glycopeptides or by searching fragmentation data (MS/MS spectra) against a database containing known peptide and glycan sequences.…”

Section: Introductionmentioning

confidence: 99%

Data-independent oxonium ion profiling of multi-glycosylated biotherapeutics

Madsen

Farutin

Lin

et al. 2018

mAbs

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The characterization of glycosylation is required for many protein therapeutics. The emergence of antibody and antibody-like molecules with multiple glycan attachment sites has rendered glycan analysis increasingly more complicated. Reliance on site-specific glycopeptide analysis is therefore necessary to fully analyze multi-glycosylated biotherapeutics. Established glycopeptide methodologies have generally utilized a priori knowledge of the glycosylation states of the investigated protein(s), database searching of results generated from data-dependent liquid chromatography–tandem mass spectrometry workflows, and extracted ion quantitation of the individual identified species. However, the inherent complexity of glycosylation makes predicting all glycoforms on all glycosylation sites extremely challenging, if not impossible. That is, only the “knowns” are assessed. Here, we describe an agnostic methodology to qualitatively and quantitatively assess both “known” and “unknown” site-specific glycosylation for biotherapeutics that contain multiple glycosylation sites. The workflow uses data-independent, all ion fragmentation to generate glycan oxonium ions, which are then extracted across the entirety of the chromatographic timeline to produce a glycan-specific “fingerprint” of the glycoprotein sample. We utilized both HexNAc and sialic acid oxonium ion profiles to quickly assess the presence of Fab glycosylation in a therapeutic monoclonal antibody, as well as for high-throughput comparisons of multi-glycosylated protein drugs derived from different clones to a reference product. An automated method was created to rapidly assess oxonium profiles between samples, and to provide a quantitative assessment of similarity.

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“…The IgA1 hinge region contains up to nine potential O-glycosylation sites clustering in a 19 amino acid peptide sequence 29 . A variety of MS analytical approaches have been used to characterize the glycan heterogeneity present in this portion of the immunoglobulin with only moderate success 30–33 . Additionally, IgA1 O-glycan site localization has been reported combining different protease digestions and ECD/ETD 29, 32, 33 .…”

Section: Introductionmentioning

confidence: 99%

Site-Specific Glycosylation of Secretory Immunoglobulin A from Human Colostrum

et al. 2015

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Secretory Immunoglobulin A (sIgA) is a major glycoprotein in milk and plays a key role in mediating immune protection of the gut mucosa. Although it is a highly glycosylated protein, its site-specific glycosylation and associated glycan micro-heterogeneity has still not been fully elucidated. In this study, the site-specific glycosylation of sIgA isolated from human colostrum (n = 3) was analyzed using a combination of LC/MS and LC/MS/MS and in-house software (Glycopeptide Finder). The majority of the glycans found are bi-antennary structures with one or more acidic Neu5Ac residue, however a large fraction belonged to truncated complex structures with terminal GlcNAc. Multiple glycosites were identified with nearly 30 glycan compositions located at seven sites on the secretory component, six compositions at a single site on the J-chain, and 16 compositions at five sites on the IgA heavy (H) chain. Site-specific heterogeneity and relative quantitation of each composition and the extent of occupation at each site was determined using non-specific proteases. Additionally, 54 O-linked glycan compositions located at the IgA1 hinge region (HR) were identified by comparison against a theoretical O-glycopeptide library. This represents the most comprehensive report to date detailing the complexity of glycan micro-heterogeneity with relative quantitation of glycoforms for each glycosylation site on milk sIgA. This strategy further provides a general method for determining site-specific glycosylation in large protein complexes.

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Clustered O-Glycans of IgA1

Cited by 91 publications

References 53 publications

The Combined Role of Galactose-Deficient IgA1 and Streptococcal IgA–Binding M Protein in Inducing IL-6 and C3 Secretion from Human Mesangial Cells: Implications for IgA Nephropathy

The Combined Role of Galactose-Deficient IgA1 and Streptococcal IgA–Binding M Protein in Inducing IL-6 and C3 Secretion from Human Mesangial Cells: Implications for IgA Nephropathy

Data-independent oxonium ion profiling of multi-glycosylated biotherapeutics

Site-Specific Glycosylation of Secretory Immunoglobulin A from Human Colostrum

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