抄録
We reported previously that the major effector cells essential for allograft (e.g., BALB/c skin and Meth A tumor; both H-2Dd) rejection were allograft-induced macrophages (AIM; H-2Db) and that AIM exhibited the cytotoxic activity against the allograft with MHC haplotype specificity. In the last meeting, we reported that we isolated a cDNA clone, 15-4-4 (261-bp fragment), by the expression cloning method using a monoclonal antibody, R15, specific for AIM and an H-2Dd tetramer. In the present study, we further characterized the cDNA. In order to know whether the protein encoded by 15-4-4 cDNA is functional or not, we ligated a full-length cDNA (1181-bp) with pEGFPNI vector; and the cDNA or vector alone was stably transfected into 293T cells. After selection of the transfectants by both EGFP expression and neomycin (G418) resistance, binding abilities of the expressed protein to an H-2Dd or H-2Db tetramer were examined under a confocal microscope or by cell sorter. The analyses revealed that the 293T cells transfected with full-length 15-4-4 cDNA did react with R15 antibody and H-2Dd tetramer and that the cells transfected with vector alone did not. In contrast, H-2Db tetramer did not react with 293T transfectants. These results suggest that the protein encoded by 15-4-4 cDNA may be a putative receptor for allogeneic MHC, H-2Dd. [Jpn J Physiol 55 Suppl:S68 (2005)]
