Galectin-8 in IgA Nephritis: Decreased Binding of IgA by Galectin-8 Affinity Chromatography and Associated Increased Binding in Non-IgA Serum Glycoproteins

Immunoglobulin A nephritis (IgAN) was first described in 1968 by Berger and colleagues; in an immunofluorescence study of renal biopsies from an unknown form of glomerulonephritis, mesangial deposits with IgA as their main component were found [1]. Detection of such IgA deposits in renal biopsies is still the only means to diagnose what is now recognized to be the most common glomerulonephritis worldwide, affecting 1.3% of the population [2], with 20–40% developing renal end stage failure within 20 years [3]. Population studies showing familiar clustering and geographical variations [4‐6] and genetic studies [2, 7, 8] suggest a strongly inherited predisposition for IgAN, although no causative mechanism has been identified.

Considerable evidence suggests that the IgA deposited in the kidney has originated from circulating undergalactosylated IgA1 complexes [9‐12]. Each IgA1 heavy chain contains up to six O-linked glycans in the hinge region between the CH1 and CH2 domains (Fig. 1). In normal IgA1, complete core-1 O-glycans like NeuAcα2,3Galβ1-3GalNAc linked to Ser or Thr are common (top glycan in Fig. 1), whereas in IgA nephritis IgA1, the O-glycans tend to lack the galactose residue as in GalNAc-Ser(Thr) or NeuAcα2,6GalNAc-Ser(Thr) (two bottom glycans in Fig. 1). In IgA nephritis, IgA-producing B cells have a glycosyltransferase imbalance in which a β1,3 galactosyltransferase and/or its chaperone Cosmc is downregulated [13, 14], resulting in decreased formation of Galβ1-3GalNAc (second glycan in Fig. 1), and increased activity of a α2,6 sialyltransferase resulting in increased addition of NeuAcα2,6 to the GalNAc (bottom glycan of Fig. 1) that also prevents further addition of Galβ1,3; the absent galactose in turn prevents further addition of NeuAcα2,3. Genetic variants of the β1,3 galactosyltransferase (C1GalT1) and its chaperone Cosmc with decreased activity and the α2,6 sialyltransferase with increased activity [15] may contribute to this and thereby predispose to IgA nephritis, but there may also be other non-genetic mechanisms for the aberrant glycosylation of IgA.

Evidence from many studies suggest that the abnormal O-glycosylation of IgA1 found in IgAN patients plays a central role in the pathogenesis of the disease [11, 14, 16, 17], but the mechanism remains unclear [18, 19]. Altered aggregation, altered interaction with mesangial cells in the kidney, altered binding to IgA receptors, and IgG-specific recognition for exposed GalNAc all have been suggested to contribute either to increased deposition of IgA-containing complexes in the kidney or decreased clearance in the liver. Altered interaction with a carbohydrate-binding protein, a lectin, would be a reasonable hypothesis to explain the changed function of undergalactosylated IgA. Snail lectins specifically binding the exposed GalNAc residues have been used diagnostically for detection in patients [20, 21], but there have been few studies on the relationship of IgA glycosylation and the binding of endogenous lectins that might affect its function.

Galectin-8 is a good candidate for such a relationship. Galectin-8 contains two canonical galectin carbohydrate recognition domains (CRD) joined by a linker [22]. Like other galectin CRDs, they bind β-galactosides, but the N-terminal CRD of galectin-8 (galectin-8N) has a particularly high affinity if the β-galactoside is 2–3-sialylated and also bound with a 1–3 linkage to the next sugar, as found in NeuAcα2,3Galβ1,3GalNAc (top glycan of Fig. 1) [23, 24], and is the only mammalian galectin with high affinity for IgA [25]. In addition, a NeuAcα2,6 attached to the GalNAc residue strongly reduces affinity for galectin-8N [24]. This predicts that the carbohydrate structural and enzymatic changes in IgA nephritis patients described in the previous paragraph should reduce the binding of IgA1 to galectin-8N. In addition to this, galectin-8 exerts several immunoregulatory functions, playing a critical role in shaping the immune response and regulating inflammation [26, 27]. Depending on the context, galectin-8 can provide both inhibitory and stimulatory effects on immune cell adhesion [28, 29], in addition to induction of immune cell growth and apoptosis [30, 31]. In contrast to cytokines, galectins do not bind specific individual receptors, but rather “sense” the glycocode expressed on the cell surface of a cell. The dual activities of galectin-8 may therefore reflect a controlled regulation of glycosylation, e.g., activation and differentiation of immune cells but could also be a consequence of disease-associated glycosylation changes, e.g., immune escape mechanisms in which cell surface glycans can be altered to avoid immune recognition. For instance, we have recently found that sera from metastatic breast cancer patients contain two to three times more galectin-1 ligands and that this glycosylation change may result in altered function relevant for the disease [32]. In relation to the present study, using an autoimmune model of rheumatoid arthritis, galectin-8 has been shown to be trapped in the inflamed joint prohibiting it from inducing apoptosis in inflammatory cells resulting in an enhanced inflammatory response [33]. In light of these considerations, analyzing galectin-8 ligands in sera from IgAN patients has a great potential to not only detect the known alterations in glycosylation of the disease but may also suggest a pathophysiologically relevant function since these ligands most likely will encounter this galectin in tissue cells.