Consistent with the co-expression of NB1 and PR3 on the same cell

Consistent with the co-expression of NB1 and PR3 on the same cell, a larger percentage of mNB1-expressing neutrophils was a risk factor for ANCA vasculitis [27]. The role of the lacking PR3–NB1 interaction in mice could be one reason

for the difficulty in generating U0126 purchase an anti-PR3 antibody-mediated disease model, and needs further study. We have reviewed the data describing modes of ANCA antigen expression on the neutrophil membrane and how ANCA can bind to their targets on the plasma membrane to initiate activation. Also conceivable is the possibility that ANCA internalization by the neutrophil contributes to activation. In fact, ANCA penetration into neutrophils has been observed by different investigators; however, the mechanisms and significance of this observation for the activation process are

not yet understood CH5424802 manufacturer [9,28,29]. Furthermore, reactivation of PR3 and MPO transcription has been observed and epigenetic mechanisms that control this process are beginning to be characterized [30,31]. It will be interesting to see if this process results in a protein or cellular localization distinct from those of the ‘original’ PR3 antigen. An additional ANCA target is the lysosomal membrane glycoprotein lysosomal-associated membrane protein 2 (LAMP-2) that was implicated in pauci-immune necrotizing glomerulonephritis by Kain et al. [32,33]. LAMP-2 is a heavily glycosylated protein expressed in many cell types, including neutrophils and endothelial cells. Lysosomal membrane proteins were detected in membranes of different cellular compartments such as lysosomes, multi-vesicular bodies, the trans-Golgi and plasma membranes [34]. LAMP-2 was found mainly in granule membranes of resting neutrophils and its plasma

membrane expression was increased with fMLF treatment [32]. The clinical significance of LAMP-2 as an ANCA antigen in small vessel vasculitis was challenged by the Chapel Hill group. The investigators filipin found much lower anti-LAMP antibody titres compared with antibodies to PR3 and MPO, no correlation with vasculitis disease activity and no disease induction by passive antibody transfer into rats [35]. Kain et al. were able, very recently, to repeat their findings in different European patient cohorts [36]. The conflicting data have no obvious explanation, but may be related to methodological and population differences as discussed by Flint et al. [37]. Major findings with respect to ANCA antigens are summarized in Fig. 1. Once ANCA have bound their neutrophil-expressed antigens, signalling and activation are initiated. Several investigators have characterized the part of the ANCA molecule that is important for neutrophil activation. Conflicting data exist, but the emerging picture is that both the antigen-binding part and the Fc part are needed. We found that ANCA Fab bind to their antigens expressed on the neutrophil, but did not trigger activation.

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