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. 2009 Jun 25;4(6):e6044. doi: 10.1371/journal.pone.0006044

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Kim et al.

This is an open-access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are properly credited.

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(A) Wild type (WT), CD28^−/−, and LFA-1^−/− 2C T cells, pre- treated with the respective mAbs, were cultured with or without the peptide-loaded L^dB7-1ICAM-1 pMVs, as indicated, followed by mAb staining for B7-1 and flow cytometric analysis. Mean fluorescence intensities (MFIs) of B7-1 staining relative to that of WT 2C T cells, pre-treated with control mAb and cultured with the QL9-loaded pMVs, were plotted. Note that P1A peptide forms complex with L^d but L^d/P1A complex is not recognized by 2C TCR [8]. (B) WT 2C T cells, pre-treated with the respective mAbs, were cultured with the peptide-loaded pMVs for different periods of time, as indicated, and stained for B7-1. (C) WT 2C T cells were treated with PP2 (PP), Wortmannin (WM), Pervanadate (PV), Cytochalasin D (CT), BAPTA/AM (BA), Forskolin (FS), Cyclosporin A (CC) and Nocodazole (NZ), respectively, as indicated, before culture with the QL9-loaded pMVs. MFIs of the B7-1 staining relative to that of 2C T cells treated with DMSO alone were plotted.