The specificity of this observation was underlined by control experiments, in which the use of serum from mice sensitized
against a different antigen did not result in increased T-cell activation when FcR γ-chain deficient DC were used. This largely excludes the possibility that circulating inflammatory factors, such as amyloid P or C reactive protein 26, in sensitized this website mice could account for the results. Furthermore, it confirms that FcγRI, FcγRIII or FcγRIV are required for augmented antigen presentation and also that lung DC lacking these receptors are devoid of constitutively defective processing or presentation via MHC class II. Considering that OVA-specific IgG1 is generated during sensitization 13 and given the fact that IgG1 binding by activating FcγR is exclusively dependent on FcγRIII 27–29, with no contribution of FcγRI and FcγRIV 11, 30, we speculate that FcγRIII is the major mediator of these effects. Further
studies using targeted knock down of FcγR on Selleck ABT 888 DC after sensitization or Th2 cell transfer might help to further delineate the function and contribution of these effects to pulmonary hypersensitivity. We assumed that under physiological conditions the formation of immune complexes would have a preferential impact on activation and antigen presentation of lung DC 17, 18 and thus examined DC outside secondary lymphoid organs. Further studies are required in order to identify specific lung DC subsets that might be involved in this process
28 and to investigate whether other Fc-receptor expressing cells contribute to this effect. It seems likely that migratory and resident LN DC populations could be regulated through IgG in a similar way. This would have important Galeterone implications, not only for the priming of antigen-specific allergic T-cell responses and the re-challenge of existing T-cell populations, but presumably also on the collateral priming to inhaled antigens 4. In this respect, the DC activation and cytokine production following engagement of activatory FcγR could be of further relevance. It is important to note, however, that allergen-specific IgG can also alleviate the strength of a pulmonary hypersensitivity reaction, presumable by modulationg macrophage function through FcγR 31. In summary, we conclude that not only IgE but also IgG and FcγR play an important role during the manifestation of allergen-induced airway hyperresponsiveness and inflammation. In addition to their function during sensitization against allergens, FcγR-mediated enhanced antigen presentation and T-cell stimulation by lung DC appears to have a significant impact on inflammatory responses during the airway challenge phase. These data support therapeutic strategies that target FcγR for the treatment of asthma.