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1 (DTT) showed that the majority of remaining lymphocytotoxicity against GalT-KO swine was mediated by
3 Screening was done by complement-dependent lymphocytotoxicity and antihuman globulin augmentation t
5 onsiveness was demonstrated by cell-mediated lymphocytotoxicity and mixed lymphocyte response, and su
6 xed lymphocyte reaction (MLR), cell-mediated lymphocytotoxicity, and cytokine profile of unresponsive
7 fractoriness in longitudinal panels from 170 lymphocytotoxicity assay (LCA)(-) and 20 LCA(+) TRAP par
8 sms to sensitize appropriate target cells in lymphocytotoxicity assays and found that the MTF is deri
9 g 29 patients, FCXM and complement-dependent lymphocytotoxicity assays were performed 10+/-2 and 28+/
10 ytotoxic cross-matches (complement-dependent lymphocytotoxicity assays) were stratified on the basis
11 on of the four methods, complement-dependent lymphocytotoxicity (CDC) and C1q-, C4d-, and IgG-Luminex
12 than was obtainable by complement-dependent lymphocytotoxicity (CDC) assays has resulted in a new pa
14 lymphocyte cultures (MLC) and cell-mediated lymphocytotoxicity (CML) culture systems analogous to th
18 ed lymphoid tissues, which resulted in acute lymphocytotoxicity, including the death of forkhead box
20 lity was determined at study entry only by a lymphocytotoxicity screening assay (s-LCA) against a pan
21 lysis is a more useful clinical parameter of lymphocytotoxicity testing than simple reporting of % PR