![DC process and present allopeptides derived from internalized exosomes. (A) Processing of exosomal alloAgs by BMDCs occurred within vesicles at low pH. Following culture of BMDCs (B10) with allogeneic exosomes (BALB/c), mature (CD86+) DCs exhibited the highest levels of IAb-IEα52-68 on the cell surface recognized by the Y-Ae mAb. NH4Cl inhibited reversibly the formation of IAb-IEα52-68 on DCs. NH4Cl did not reduce binding of IEα52-68 to IAb (not shown). Numbers indicate percentage of cells. (B) BMDCs (B10) were pulsed with graded concentrations of BALB/c exosomes or with B10 or C3H exosomes. Then, decreasing numbers of DCs were added to 105 BEα20.6 T cells specific for IAb-IEα52-68. T-cell activation was evaluated by IL-2 secretion assessed by the HT-1 cell proliferation assay. (C) Recognition of IAb-IEα52-68 by T cells was inhibited with Y-Ae mAb. IEα52-68 was used as positive control and the OVA-derived peptide SIINFEKL as irrelevant control. (D) BMDCs increased their capacity to present exosomal allopeptides to 1H3.1 TCRtg CD4+ T cells after activation via CD40. 1H3.1 T-cell proliferation was evaluated after 72 hours by [3H] TdR incorporation. Each condition was tested in triplicate and displayed as their means ± SD. Data are representative of 3 independent experiments.](https://ash.silverchair-cdn.com/ash/content_public/journal/blood/104/10/10.1182_blood-2004-03-0824/6/zh80220469510004.jpeg?Expires=1720446049&Signature=1GiVHHXo1MUqvyA-fmvN0lq8xBPjMHxphH-K4G3mZIyjIJImKVlx4dlFKKdF1VssD6rMOwNDgD7~S8HFFpx9y1ikVu0vqWYq4z4Uwn-T7D2t8a2j~EHN-HSXLxlyjvPdX9RsBkbm4XGkhJpVBh7nWjgzQF4ol74yg7YBngAgRZD6qQkE~ORiZrxdl6FIgYtqV9bHAbL6gLlYvZBgEg87H7OtDtGdbi9bXiwzd34QTi71XPxUgiak-~M0jsdWhN~H2deuj2rR--QEp16AOBLGDcdjHfUT48EXdr5iZsWFFPBzMtgcHiX9crBeT94bFwqd9wo94yG7drugwCDQo8~-KQ__&Key-Pair-Id=APKAIE5G5CRDK6RD3PGA)
DC process and present allopeptides derived from internalized exosomes. (A) Processing of exosomal alloAgs by BMDCs occurred within vesicles at low pH. Following culture of BMDCs (B10) with allogeneic exosomes (BALB/c), mature (CD86+) DCs exhibited the highest levels of IAb-IEα52-68 on the cell surface recognized by the Y-Ae mAb. NH4Cl inhibited reversibly the formation of IAb-IEα52-68 on DCs. NH4Cl did not reduce binding of IEα52-68 to IAb (not shown). Numbers indicate percentage of cells. (B) BMDCs (B10) were pulsed with graded concentrations of BALB/c exosomes or with B10 or C3H exosomes. Then, decreasing numbers of DCs were added to 105 BEα20.6 T cells specific for IAb-IEα52-68. T-cell activation was evaluated by IL-2 secretion assessed by the HT-1 cell proliferation assay. (C) Recognition of IAb-IEα52-68 by T cells was inhibited with Y-Ae mAb. IEα52-68 was used as positive control and the OVA-derived peptide SIINFEKL as irrelevant control. (D) BMDCs increased their capacity to present exosomal allopeptides to 1H3.1 TCRtg CD4+ T cells after activation via CD40. 1H3.1 T-cell proliferation was evaluated after 72 hours by [3H] TdR incorporation. Each condition was tested in triplicate and displayed as their means ± SD. Data are representative of 3 independent experiments.
