![Figure 1. Identification of a DR*0401/BHRF1 epitope recognized by the CD4 T-cell clone 4.19. (A) Recognition of the lytic EBV protein BHRF1 by clone 4.19. CTL cells were tested in a 4-hour TNF-α release assay on autologous B-LCLs expressing individual latent or lytic EBV proteins from vaccinial viral vectors. Results are shown as μg/mL. TNF release was observed at an effector-target ratio of 10:1. (B) Identification of the target epitope of BHRF1-specific clone 4.19 using a panel of peptides (23-mers, overlapping by 12 amino acids [aa's]) spanning the BHRF1 protein. These peptides were used as targets in cytotoxic assays by incubating them with 51Cr-labeled autologous EBV-B cells for 1 hour at 37°C. Clone 4.19 was added at an E/T ratio of 10:1 and Cr release was measured after 4 hours. Note the significant lysis background observed with unloaded autologous B-LCL (No pep). (C) Stimulation of clone 4.19 by the BHRF1 122-133 peptide (PYY). Cytotoxicity of clone 4.19 to Cr-labeled autologous EBV-B cells loaded with various concentrations of peptides. Clone 4.19 was added at an E/T ratio of 10:1 and Cr release was measured after 4 hours. Data obtained with the 23-mer BHRF1111-133 peptide are shown as a positive control. Data obtained with an irrelevant peptide (irr peptide) are shown as a negative control.](https://ash.silverchair-cdn.com/ash/content_public/journal/blood/103/4/10.1182_blood-2003-03-0930/6/zh80040456650001.jpeg?Expires=1724977381&Signature=uIBq-xo2waaUpWLYC0S5uWrP9lbS6YA8z-gG8YXLEIKrYaTAPT64mKJCQq~-W-3Nmibbo46N1JEADMxHaaGR0w0vh-DyIbOkBUn4v2Kuqiu8qMUtjdXF657SQpwnISlDlJ85cFL2A78Cwij9MxKWpupSvK5ln2TVU6scCPZE5rWRPknH6y-Bb7MdZS0kVXqoETThhVuPwPo7D62o9iaZW~iapSWJqawE57hgtZsFsiGjE~OX5TiY~JzDNwyfAe2iz~EW~l679wUtn05uIdkMIpn1rZxEBn5rmTxPzo1tWp0Vec82X6DPPZbVTVezdRI2QnDtC-LO8M7sj2mXD2siyg__&Key-Pair-Id=APKAIE5G5CRDK6RD3PGA)
Identification of a DR*0401/BHRF1 epitope recognized by the CD4 T-cell clone 4.19. (A) Recognition of the lytic EBV protein BHRF1 by clone 4.19. CTL cells were tested in a 4-hour TNF-α release assay on autologous B-LCLs expressing individual latent or lytic EBV proteins from vaccinial viral vectors. Results are shown as μg/mL. TNF release was observed at an effector-target ratio of 10:1. (B) Identification of the target epitope of BHRF1-specific clone 4.19 using a panel of peptides (23-mers, overlapping by 12 amino acids [aa's]) spanning the BHRF1 protein. These peptides were used as targets in cytotoxic assays by incubating them with 51Cr-labeled autologous EBV-B cells for 1 hour at 37°C. Clone 4.19 was added at an E/T ratio of 10:1 and Cr release was measured after 4 hours. Note the significant lysis background observed with unloaded autologous B-LCL (No pep). (C) Stimulation of clone 4.19 by the BHRF1 122-133 peptide (PYY). Cytotoxicity of clone 4.19 to Cr-labeled autologous EBV-B cells loaded with various concentrations of peptides. Clone 4.19 was added at an E/T ratio of 10:1 and Cr release was measured after 4 hours. Data obtained with the 23-mer BHRF1111-133 peptide are shown as a positive control. Data obtained with an irrelevant peptide (irr peptide) are shown as a negative control.
