Proteinase 3

The conformation of PR3 is essential for its reactivity with PR3-ANCA. PR3 is a linear polypeptide containing 228 amino acids. In 1994, linear epitopes of PR3 were found, and these seemed to occur in regions close to the active site of the enzyme where 4 of 5 epitopes are assumed to be located. The crystal structure of PR3 was resolved in 1996. PR3 is progressively more strongly expressed from the stage of early myelocyte maturation to the fully developed neutrophil. The gene encoding PR3 is located close to the HLE site on chromosome 19.

Myeloperoxidase

MPO is the main antigen for the P-ANCA reactivity in patients with AAV. The enzyme catalyzes the hydrogen peroxide–mediated peroxidation of chloride ions to hypochlorite, and the hypochlorous acid is effective in killing phagocytized bacteria and viruses. However, the hypochlorous acid can also inactivate proteinase inhibitors in blood and tissues, thus indirectly influencing inflammation through induction of highly reactive oxygen radical species among other mechanisms. MPO is a hydrophilic and positively charged molecule located in azurophilic and primary granules. Thus, after fixation of neutrophils and monocytes by ethanol for use as substrate in IIF, the positively charged molecule migrates toward the nucleus and the ensuing staining pattern becomes perinuclear as shown in Fig. 2 .

MPO consists of 2 polypeptides of 467 and 113 amino acids, called the α and β chains, respectively. After glycosylation and final processing, the polypeptides form a 59-kDa α chain and a 13.5-kDa β chain that are linked together in a heterodimeric 140-kDa molecule, in which each half has one α chain and one β chain. The crystal structure has been resolved, and the gene encoding MPO has been found on the long arm of chromosome 17. Reactivity with MPO-ANCA highly depends on conformational preservation of the structure. The MPO molecule is very sensitive to light exposure, whereby it cleaves at position Met 409 of the α chain, a fact that is important for its stability during purification and coating on solid phases.

Human Leukocyte Elastase

HLE is a frequently targeted autoantigen in patients with drug-induced vasculitis or drug-induced lupus and in those with cocaine-induced nasal destruction, which may mimic late-stage WG. HLE-ANCAs are rarely found alone and are mostly accompanied by ANCAs toward other neutrophil antigens.

HLE-ANCAs are rare in idiopathic AAV. If HLE-ANCA is the only ANCA contained in a serum, it gives a P-ANCA pattern.

Human Lysosomal Membrane Protein 2

Autoantibodies to a human lysosomal membrane protein (H-lamp-2) were first described in 78 of 84 individuals with ANCA-associated focal necrotizing glomerulonephritis (FNGN). Kain and colleagues reported that the H-lamp-2 protein is expressed in the plasma membrane of several human cells, such as neutrophils and ECs, but the protein is also integrated into membranes of neutrophil intracellular vesicles. A recent study from the same research group has suggested that the emergence of autoimmunity to H-lamp-2 is caused by molecular mimicry through reactivity with a H-lamp-2 peptide (P41–49) that shows 100% homology to a bacterial adhesin peptide (amino acids 72–80) found on mature FimH protein located on type 1 fimbriae of gram-negative bacteria. Xenogeneic antibodies to H-lamp-2 were found to bind to fixed neutrophils in a C-ANCA–like reaction pattern by IIF as a result of reactivity with the intracellular vesicle membranes mentioned earlier. These autoantibodies are thus not neutrophil-specific because they react with a variety of human cells, most importantly ECs, and it can be discussed whether it is justified to call them ANCA.

The H-lamp-2 protein is assumed to have physiologic roles in cell adhesion, autophagocytosis, and antigen presentation. Autoantibodies to H-lamp-2, however, may be able to induce pauci-immune FNGN per se because a monoclonal antibody to H-lamp-2 was found to induce apoptosis of microvascular endothelium when injected into rats. In addition, rats injected with rabbit antibodies to H-lamp-2 subsequently developed FNGN.

Further studies on the prevalence and levels of anti–H-lamp-2 are needed to judge the potential clinical utility of this autoantibody in monitoring patients with AAV.

Other Antigens

Lactoferrin, bactericidal permeability-increasing protein, azurocidin, and lysozyme, which are also localized in neutrophil granules, may in some cases be targets of NSAs; however, such reactivity is rare in idiopathic small vessel necrotizing vasculitis. In contrast, any of these antigens may be a target in patients suffering from drug-induced vasculitis or drug-induced lupus-like syndromes. In these cases, there are often multiple granule protein targets, a finding so characteristic that a drug-induced syndrome should be suspected whenever multispecific ANCAs are found in serum. Sera from such patients can additionally harbor autoantibodies to histones and β ₂ -glycoprotein I, especially if the syndrome has been caused by an antithyroid drug.

Proteinase 3

The conformation of PR3 is essential for its reactivity with PR3-ANCA. PR3 is a linear polypeptide containing 228 amino acids. In 1994, linear epitopes of PR3 were found, and these seemed to occur in regions close to the active site of the enzyme where 4 of 5 epitopes are assumed to be located. The crystal structure of PR3 was resolved in 1996. PR3 is progressively more strongly expressed from the stage of early myelocyte maturation to the fully developed neutrophil. The gene encoding PR3 is located close to the HLE site on chromosome 19.

Myeloperoxidase

MPO is the main antigen for the P-ANCA reactivity in patients with AAV. The enzyme catalyzes the hydrogen peroxide–mediated peroxidation of chloride ions to hypochlorite, and the hypochlorous acid is effective in killing phagocytized bacteria and viruses. However, the hypochlorous acid can also inactivate proteinase inhibitors in blood and tissues, thus indirectly influencing inflammation through induction of highly reactive oxygen radical species among other mechanisms. MPO is a hydrophilic and positively charged molecule located in azurophilic and primary granules. Thus, after fixation of neutrophils and monocytes by ethanol for use as substrate in IIF, the positively charged molecule migrates toward the nucleus and the ensuing staining pattern becomes perinuclear as shown in Fig. 2 .

MPO consists of 2 polypeptides of 467 and 113 amino acids, called the α and β chains, respectively. After glycosylation and final processing, the polypeptides form a 59-kDa α chain and a 13.5-kDa β chain that are linked together in a heterodimeric 140-kDa molecule, in which each half has one α chain and one β chain. The crystal structure has been resolved, and the gene encoding MPO has been found on the long arm of chromosome 17. Reactivity with MPO-ANCA highly depends on conformational preservation of the structure. The MPO molecule is very sensitive to light exposure, whereby it cleaves at position Met 409 of the α chain, a fact that is important for its stability during purification and coating on solid phases.

Human Leukocyte Elastase

HLE is a frequently targeted autoantigen in patients with drug-induced vasculitis or drug-induced lupus and in those with cocaine-induced nasal destruction, which may mimic late-stage WG. HLE-ANCAs are rarely found alone and are mostly accompanied by ANCAs toward other neutrophil antigens.

HLE-ANCAs are rare in idiopathic AAV. If HLE-ANCA is the only ANCA contained in a serum, it gives a P-ANCA pattern.

Human Lysosomal Membrane Protein 2

Autoantibodies to a human lysosomal membrane protein (H-lamp-2) were first described in 78 of 84 individuals with ANCA-associated focal necrotizing glomerulonephritis (FNGN). Kain and colleagues reported that the H-lamp-2 protein is expressed in the plasma membrane of several human cells, such as neutrophils and ECs, but the protein is also integrated into membranes of neutrophil intracellular vesicles. A recent study from the same research group has suggested that the emergence of autoimmunity to H-lamp-2 is caused by molecular mimicry through reactivity with a H-lamp-2 peptide (P41–49) that shows 100% homology to a bacterial adhesin peptide (amino acids 72–80) found on mature FimH protein located on type 1 fimbriae of gram-negative bacteria. Xenogeneic antibodies to H-lamp-2 were found to bind to fixed neutrophils in a C-ANCA–like reaction pattern by IIF as a result of reactivity with the intracellular vesicle membranes mentioned earlier. These autoantibodies are thus not neutrophil-specific because they react with a variety of human cells, most importantly ECs, and it can be discussed whether it is justified to call them ANCA.

The H-lamp-2 protein is assumed to have physiologic roles in cell adhesion, autophagocytosis, and antigen presentation. Autoantibodies to H-lamp-2, however, may be able to induce pauci-immune FNGN per se because a monoclonal antibody to H-lamp-2 was found to induce apoptosis of microvascular endothelium when injected into rats. In addition, rats injected with rabbit antibodies to H-lamp-2 subsequently developed FNGN.

Further studies on the prevalence and levels of anti–H-lamp-2 are needed to judge the potential clinical utility of this autoantibody in monitoring patients with AAV.

Other Antigens

Lactoferrin, bactericidal permeability-increasing protein, azurocidin, and lysozyme, which are also localized in neutrophil granules, may in some cases be targets of NSAs; however, such reactivity is rare in idiopathic small vessel necrotizing vasculitis. In contrast, any of these antigens may be a target in patients suffering from drug-induced vasculitis or drug-induced lupus-like syndromes. In these cases, there are often multiple granule protein targets, a finding so characteristic that a drug-induced syndrome should be suspected whenever multispecific ANCAs are found in serum. Sera from such patients can additionally harbor autoantibodies to histones and β ₂ -glycoprotein I, especially if the syndrome has been caused by an antithyroid drug.