Chronic inflammatory demyelinating polyneuropathy (CIDP): change of serum IgG dimer levels during treatment with intravenous immunoglobulins

We first analyzed the dimer content in serum IgG fractions before (pre) and after (post) IVIg infusion in patients with CIDP, MG, and MFS. Dimeric IgG fractions could be detected in most serum samples and varied between 0 and 11.3 % of total IgG (Fig. 1a, b). In CIDP patients, there was no association between IgG dimer levels pre- and post-IVIg treatment and age, body weight, or disease severity. IgG dimer levels were significantly higher in post- compared to pre-infusion samples (dimer content pre-IVIg 2.6 % ± 1.5, post-IVIg 5.8 % ± 2.9, Fig. 1c). We also measured the percentage of IgG dimers in five controls and found similar IgG dimer levels compared to CIDP patients (dimer content 2.4 ± 1.3 %). Further, we assessed the dimer content in different lots of two commercial IVIg preparations (Privigen®, CSL Behring and Gamunex®, Grifols) that were used in our patients and found higher values (4.0 % ± 2.3 and 4.9 % ± 1.5, respectively) compared to the average percentage in healthy controls and pre-treatment serum samples from CIDP patients.

To assess the utility of IgG dimer levels as a surrogate marker for treatment response to IVIg, we grouped our cohort of CIDP patients according to their clinical response to IVIg treatment (stable/improving vs. worsening) and calculated the change of IgG dimer values in those two groups. CIDP patients who showed improvement or stabilization of the disease course during IVIg treatment (n = 13) had significantly elevated post-IgG dimer levels compared to those who worsened under IVIg treatment (n = 3, Fig. 1d). This difference could be detected irrespective which of the two available IVIg preparations were used (Fig. 1e, f).

There is strong experimental evidence that IgG dimers, which are detectable in pooled human IgG fractions from different individuals, consist of Id-anti-Id antibody pairs. Therefore, it is likely that in CIDP, post-treatment IgG dimers may also contain Id-autoantibodies and their anti-idiotypes. This hypothesis cannot be directly validated in CIDP, since the target antigens of the presumed autoantibodies in CIDP are unknown.

To further characterize the nature of IgG dimers that emerge after IVIg infusion, we collected monomeric and dimeric IgG peaks from two patients with MFS and from one patient with MG who were treated with IVIg. Patients #1 and #2 were seropositive for anti-GQ1b IgG antibodies, and patient #3 had serum IgG antibodies against acetylcholine receptors (71 nmol/l). We anticipated that IVIg dimers, which occur after IVIg treatment as a result of Id-anti-Id binding, should contain measurable amounts of those autoantibodies. Therefore, we re-monomerized the dimer fraction by dialyzing against 10 mM acetic acid at pH 4.0 and tested pre-IVIg treatment monomeric IgG and post-IVIg treatment monomeric and dimeric IgG fractions for immune reactivity against GQ1b and AchR, respectively. Monomeric and dimeric IgG fractions of the patient with myasthenia displayed reactivity against AchR (pre-monomeric 969 ± 10.1 cpm, post-dimeric 127 ± 6.5 cpm, post-monomeric 547.2 ± 16 cpm). Reactivity against GQ1b could be shown in monomeric IgG fractions pre- and post-IVIg treatment as well as to a higher extent in dimeric IgG fraction post-IVIg treatment (Fig. 2), suggesting that IgG dimers which occur after IVIg treatment in those two patients are formed by complexes that include autoantibodies and their presumed anti-idiotypes in IVIg preparations.

Based on our experiments using GQ1b and AchR antibody-positive sera, we further anticipated that IgG dimers that occur after IVIg treatment in CIDP patients may also contain autoantibodies and their IVIg-derived anti-idiotypes. We therefore used post-IVIg treatment-derived IgG dimers for screening for autoimmune reactivity against neuronal or Schwann cell epitopes in peripheral nerve fibers. Four out of ten tested dimeric IgG samples stained axons and/or myelin of peripheral nerve fibers (Fig. 3).

This immunofluorescence was not detected in monomeric or dimeric IVIg fractions, pre-dimeric IgG, or from post-dimeric IgG derived from patients with MFS or MG. Pre-treatment of tissue samples with methanol/chloroform abrogated staining with dimeric IgG, indicating that those epitopes are membrane associated. From these data, we conclude that dimeric IgG contains antibodies that may recognize epitopes expressed on peripheral axons and Schwann cells.